EP2354161B1 - Anti-nr10 antibody, and use thereof - Google Patents

Anti-nr10 antibody, and use thereof Download PDF

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EP2354161B1
EP2354161B1 EP09830463.7A EP09830463A EP2354161B1 EP 2354161 B1 EP2354161 B1 EP 2354161B1 EP 09830463 A EP09830463 A EP 09830463A EP 2354161 B1 EP2354161 B1 EP 2354161B1
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seq
amino acid
acid sequence
antibody
antibodies
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EP2354161A4 (en
EP2354161A1 (en
Inventor
Taichi Kuramochi
Keiko Kasutani
Souhei Ohyama
Hiroyuki Tsunoda
Tomoyuki Igawa
Tatsuhiko Tachibana
Hirotake Shiraiwa
Keiko Esaki
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Chugai Pharmaceutical Co Ltd
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Chugai Pharmaceutical Co Ltd
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Priority claimed from PCT/JP2008/072152 external-priority patent/WO2009072604A1/ja
Priority claimed from PCT/JP2009/054941 external-priority patent/WO2010064456A1/ja
Application filed by Chugai Pharmaceutical Co Ltd filed Critical Chugai Pharmaceutical Co Ltd
Priority to EP15172595.9A priority Critical patent/EP2949672A1/en
Priority to SI200931302T priority patent/SI2354161T1/sl
Priority to PL09830463T priority patent/PL2354161T3/pl
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    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K16/00Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
    • C07K16/18Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans
    • C07K16/28Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against receptors, cell surface antigens or cell surface determinants
    • C07K16/2866Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against receptors, cell surface antigens or cell surface determinants against receptors for cytokines, lymphokines, interferons
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P29/00Non-central analgesic, antipyretic or antiinflammatory agents, e.g. antirheumatic agents; Non-steroidal antiinflammatory drugs [NSAID]
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
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    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K16/00Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
    • C07K16/18Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans
    • C07K16/28Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against receptors, cell surface antigens or cell surface determinants
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/505Medicinal preparations containing antigens or antibodies comprising antibodies
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    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/20Immunoglobulins specific features characterized by taxonomic origin
    • C07K2317/24Immunoglobulins specific features characterized by taxonomic origin containing regions, domains or residues from different species, e.g. chimeric, humanized or veneered
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    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/50Immunoglobulins specific features characterized by immunoglobulin fragments
    • C07K2317/56Immunoglobulins specific features characterized by immunoglobulin fragments variable (Fv) region, i.e. VH and/or VL
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/50Immunoglobulins specific features characterized by immunoglobulin fragments
    • C07K2317/56Immunoglobulins specific features characterized by immunoglobulin fragments variable (Fv) region, i.e. VH and/or VL
    • C07K2317/565Complementarity determining region [CDR]
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/50Immunoglobulins specific features characterized by immunoglobulin fragments
    • C07K2317/56Immunoglobulins specific features characterized by immunoglobulin fragments variable (Fv) region, i.e. VH and/or VL
    • C07K2317/567Framework region [FR]
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/70Immunoglobulins specific features characterized by effect upon binding to a cell or to an antigen
    • C07K2317/76Antagonist effect on antigen, e.g. neutralization or inhibition of binding
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/90Immunoglobulins specific features characterized by (pharmaco)kinetic aspects or by stability of the immunoglobulin
    • C07K2317/92Affinity (KD), association rate (Ka), dissociation rate (Kd) or EC50 value
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2317/00Immunoglobulins specific features
    • C07K2317/90Immunoglobulins specific features characterized by (pharmaco)kinetic aspects or by stability of the immunoglobulin
    • C07K2317/94Stability, e.g. half-life, pH, temperature or enzyme-resistance

Definitions

  • the present invention relates to anti-NR10 antibodies, and pharmaceutical compositions comprising an anti-NR10 antibody.
  • cytokines are known as humoral factors involved in the growth and differentiation of various types of cells, or in the activation of differentiated mature cell functions. Cytokine-stimulated cells produce different types of cytokines, thereby forming networks of multiple cytokines in the body. Biological homeostasis is maintained by a delicate balance of the mutual regulation between cytokines in these networks. Many inflammatory diseases are thought to result from a failure of such cytokine networks. Thus, monoclonal antibody-based anti-cytokine therapy is drawing much attention. For example, anti-TNF antibodies and anti-IL-6 receptor antibodies have been demonstrated to be highly effective clinically. On the other hand, there are many examples of failure where no therapeutic effects were produced when a single cytokine, such as IL-4, was blocked alone, due to the activation of compensatory pathways in actual pathological conditions.
  • the present invention succeeded in isolating a novel cytokine receptor NR10 that was highly homologous to gpl30, a receptor for IL-6 signal transduction (Patent Document 1).
  • NR10 forms a heterodimer with, oncostatin M receptor (OSMR) and functions as an IL-31 receptor (Non-patent Document 1).
  • OSMR oncostatin M receptor
  • IL-31 it has been reported that transgenic mice overexpressing IL-31 spontaneously develop pruritic dermatitis (Patent Document 2).
  • Antibodies that bind to NR10 and inhibit the binding between NR10 and IL-31 may be effective in treating inflammatory diseases.
  • anti-NR10 antibodies are required to have low immunogenicity.
  • antibodies with strong NR10-binding or neutralizing activity are desired.
  • mouse anti-NR10 neutralizing antibodies for use in the treatment of inflammatory diseases were described (Patent Document 3).
  • An objective of the present invention is to provide anti-NR10 antibodies, and pharmaceutical compositions comprising an anti-NR10 antibody.
  • the present inventors conducted dedicated studies to achieve the objective described above.
  • the present inventors succeeded in obtaining anti-NR10 antibodies having an effective neutralizing activity against NR10.
  • the present inventors succeeded in humanizing the antibodies while maintaining their activity.
  • the present inventors also successfully produced antibodies with improved pharmacokinetics, enhanced antigen-binding activity, improved stability, and/or reduced risk of immunogenicity. These antibodies are useful as therapeutic agents for inflammatory diseases.
  • the present invention relates to anti-NR10 antibodies, and pharmaceutical compositions comprising an anti-NR10 antibody. More specifically, the present invention includes:
  • NR10 is a protein that forms a heterodimer with oncostatin M receptor (OSMR) and functions as an IL-31 receptor.
  • OSMR oncostatin M receptor
  • NR10 is also known as glm-r ( J Biol Chem 277, 16831-6, 2002 ), GPL ( J Biol Chem 278, 49850-9, 2003 ), IL31RA ( Nat Immunol 5, 752-60, 2004 ), and such.
  • NR10 as disclosed herein also includes proteins called by such names.
  • NR10 also referred to as IL31RA, GPL, or glm-r
  • IL31RA also referred to as GPL, or glm-r
  • NR10 derived from humans, mice, and monkeys is preferred, and human-derived NR10 is particularly preferred.
  • NR10.1 consists of 662 amino acids and contains a transmembrane domain.
  • NR10.2 is a soluble receptor-like protein consisting of 252 amino acids without the transmembrane domain.
  • known NR10 splicing variants that function as transmembrane receptor proteins include NR10.3 and IL-31RAv3.
  • the human NR10 as disclosed herein is not particularly limited, as long as it forms a heterodimer with oncostatin M receptor (OSMR) and functions as an IL-31 receptor.
  • OSMR oncostatin M receptor
  • NR10 includes NR10.3 (also referred to as ILRAv4 ( Nat Immunol 5,752-60, 2004 )) and IL-31RAv3.
  • NR 10.3 IL31RAv4
  • IL31RAv3 consists of 732 amino acids (GenBank Accession No: NM_139017).
  • the amino acid sequence of IL31RAv4 is shown in SEQ ID NO: 79
  • the amino acid sequence of IL31RAv3 is shown in SEQ ID NO: 80.
  • mouse-derived NR10 includes proteins comprising the amino acid sequence of SEQ ID NO: 81.
  • cynomolgus monkey-derived NR10 includes proteins comprising the amino acid sequence of SEQ ID NO: 66.
  • Preferred anti-NR10 antibody as disclosed herein include the anti-NR10 antibodies of any one of (1) to (8) in (A) to (D) below.
  • Substitution of Ile at position 3 in the heavy chain CDR1 of SEQ ID NO: 9 with another amino acid is not particularly limited but preferred examples thereof include Val.
  • Substitution of Met at position 4 in the heavy chain CDR1 of SEQ ID NO: 9 with another amino acid is not particularly limited but preferred examples thereof include Ile.
  • Substitution of Met at position 4 in the heavy chain CDR1 of SEQ ID NO: 9 with another amino acid is not particularly limited but preferred examples thereof include Leu.
  • Substitution of Ile at position 3 in the heavy chain CDR1 of SEQ ID NO: 9 with another amino acid is not particularly limited but preferred examples thereof include Ala.
  • Substitution of Leu at position 1 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Glu.
  • Substitution of Asn at position 3 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Gln at position 13 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Lys at position 14 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Gln.
  • Substitution of Lys at position 16 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Gln.
  • Substitution of Gly at position 17 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Lys and Gly at positions 16 and 17, respectively, in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples include substitution of Lys at position 16 with Gln, and Gly at position 17 with Asp.
  • Substitution of Lys, Lys, and Gly at positions 14, 16, and 17, respectively, in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples include substitution of Lys at position 14 with Gln, Lys at position 16 with Gln, and Gly at position 17 with Asp.
  • Substitution of Gln, Lys, Lys, and Gly at positions 13, 14, 16, and 17, respectively, in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples include substitution of Gln at position 13 with Asp, Lys at position 14 with Gln, Lys at position 16 with Gln, and Gly at position 17 with Asp.
  • Substitution of Ser at position 10 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Gln at position 13 in the heavy chain CDR2 of SEQ ID NO: 10 with another amino acid is not particularly limited but preferred examples thereof include Pro.
  • Substitution of Tyr at position 3 in the heavy chain CDR3 of SEQ ID NO: 11 with another amino acid is not particularly limited but preferred examples thereof include Leu.
  • Substitution of Met at position 10 in the heavy chain CDR3 of SEQ ID NO: 11 with another amino acid is not particularly limited but preferred examples thereof include Leu.
  • amino acid after substitution is not particularly limited but preferred examples thereof include Glu.
  • Substitution of Tyr at position 12 in the heavy chain CDR3 of SEQ ID NO: 11 with another amino acid is not particularly limited but preferred examples thereof include Thr and Ser.
  • the amino acid after substitution is not particularly limited but preferred examples include substitution of Met at position 10 with Leu, Asp at position 11 with Glu, and Tyr at position 12 with Thr.
  • substitution of Asp and Tyr at positions 11 and 12, respectively, in the heavy chain CDR3 of SEQ ID NO: 11 with another amino acid is not particularly limited but preferred examples include substitution of Asp at position 11 witch Glu, and Tyr at position 12 with Thr.
  • the amino acid after substitution is not particularly limited but preferred examples include substitution of Tyr at position 3 with Leu, Asp at position 11 with Glu, and Tyr at position 12 with Thr or Ser.
  • Substitution of Arg at position 1 in the light chain CDR1 of SEQ ID NO: 13 with another amino acid is not particularly limited but preferred examples thereof include Gln.
  • amino acid after substitution is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Arg and Asn at positions 1 and 5, respectively, in the light chain CDR1 of SEQ ID NO: 13 with another amino acid is not particularly limited but preferred examples include substitution of Arg at position 1 with Gln, and Asn at position 5 with Asp.
  • Substitution of Ser at position 8 in the light chain CDR1 of SEQ ID NO: 13 with another amino acid is not particularly limited but preferred examples thereof include Arg.
  • Substitution of Ser and Leu at positions 8 and 10, respectively, in the light chain CDR1 of SEQ ID NO: 13 with another amino acid is not particularly limited but preferred examples include substitution of Ser at position 8 with Arg, and Leu at position 10 with Val.
  • Substitution of Thr at position 2 in the light chain CDR1 of SEQ ID NO: 13 with another amino acid is not particularly limited but preferred examples thereof include Ala and Ser.
  • amino acid after substitution is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Lys at position 3 in the light chain CDR2 of SEQ ID NO: 14 with another amino acid is not particularly limited but preferred examples thereof include Gin.
  • Substitution of Leu at position 5 in the light chain CDR2 of SEQ ID NO: 14 with another amino acid is not particularly limited but preferred examples thereof include Glu.
  • Substitution of Lys at position 7 in the light chain CDR2 of SEQ ID NO: 14 with another amino acid is not particularly limited but preferred examples thereof include Gln and Asp.
  • Substitution of Lys, Leu, and Lys at positions 3, 5, and 7, respectively, in the light chain CDR2 of SEQ ID NO: 14 with another amino acid is not particularly limited but preferred examples include substitution of Lys at position 3 with Gln, Leu at position 5 with Glu, and Lys at position 7 with Gln.
  • Substitution of Glu at position 5 in the light chain CDR3 of SEQ ID NO: 15 with another amino acid is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Ser at position 6 in the light chain CDR3 of SEQ ID NO: 15 with another amino acid is not particularly limited but preferred examples thereof include Asp.
  • Substitution of Thr at position 9 in the light chain CDR3 of SEQ ID NO: 15 with another amino acid is not particularly limited but preferred examples thereof include Phe.
  • substitutions may be made alone, or multiple substitutions may be made in combination. Furthermore, the above substitutions may be combined with other substitutions. These substitutions can improve the antibody pharmacokinetics (retention in plasma), enhance the antigen-binding activity, improve the stability, and/or reduce the risk or immunogenicity.
  • variable regions having a combination of the above-described substitutions include, for example, heavy chain variable regions having the amino acid sequence of SEQ ID NO: 167 and light chain variable regions having the amino acid sequence of SEQ ID NO: 168.
  • antibodies having a combination of the above-described substitutions include, for example, antibodies that comprise a heavy chain variable region having the amino acid sequence of SEQ ID NO: 167 and a light chain variable region having the amino acid sequence of SEQ ID NO: 168.
  • variable regions having a combination of the above-described substitutions include, for example, the following variable regions:
  • any framework regions may be used for the above-described antibodies of (1) or (3); however, FRs derived from human are preferably used.
  • any constant regions may be used for the above-described antibodies of (1) to (8); however, constant regions derived from human are preferably used.
  • the amino acid sequence of the original FR or constant region may be used without modification, or after being modified to a different amino acid sequence by substitution, deletion, addition, and/or insertion of one or more amino acids.
  • amino acid sequence of the heavy chain of the above-described NS18 is shown in SEQ ID NO: 34 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 33. Meanwhile, the amino acid sequence of the light chain is shown in SEQ ID NO: 36 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 35.
  • amino acid sequence of the heavy chain of NS22 is shown in SEQ ID NO: 38 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 37. Meanwhile, the amino acid sequence of the light chain is shown in SEQ ID NO: 40 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 39.
  • amino acid sequence of the heavy chain of NS23 is shown in SEQ ID NO: 42 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 41. Meanwhile, the amino acid sequence of the light chain is shown in SEQ ID NO: 44 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 43.
  • amino acid sequence of the heavy chain of NS33 is shown in SEQ ID NO: 46 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 45. Meanwhile, the amino acid sequence of the light chain is shown in SEQ ID NO: 48 and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 47.
  • the "activity equivalent to that of the antibody of any one of (1) to (6)” means that the activity of binding and/or neutralizing NR10 (for example, human NR10) is equivalent.
  • the term “equivalent” means that the activity is not necessarily the same but may be enhanced or reduced as long as the activity is retained.
  • Antibodies with a reduced activity include, for example, antibodies having an activity that is 30% or more, preferably 50% or more, and more preferably 80% or more of that of the original antibody.
  • the antibodies of any one of (1) to (6) mentioned above may have a substitution, deletion, addition, and/or insertion of one or more amino acids in the amino acid sequence of the variable regions (CDR sequences and/or FR sequences), as long as the NR10-binding and/or neutralizing activity is retained.
  • Methods well known to those skilled in the art to prepare the amino acid sequence of an antibody that has a substitution, deletion, addition, and/or insertion of one or more amino acids in the amino acid sequence and retains NR10-binding and/or neutralizing activity include methods for introducing mutations into proteins.
  • mutants functionally equivalent to the antibody having NR10-binding and/or neutralizing activity by introducing appropriate mutations into the amino acid sequence of the antibody having NR10-binding and/or neutralizing activity using site-directed mutagenesis ( Hashimoto-Gotoh, T, Mizuno, T, Ogasahara, Y, and Nakagawa, M. (1995)
  • site-directed mutagenesis Hashimoto-Gotoh, T, Mizuno, T, Ogasahara, Y, and Nakagawa, M. (1995)
  • amino acid side chain properties are: hydrophobic amino acids (A, I, L, M, F, P, W, Y, and V), hydrophilic amino acids (R, D, N, C, E, Q, G, H, K, S, and T), amino acids containing aliphatic side chains (G, A, V, L, I, and P), amino acids containing hydroxyl group-containing side chains (S, T, and Y), amino acids containing sulfur-containing side chains (C and M), amino acids containing carboxylic acid- and amide-containing side chains (D, N, E, and Q), amino acids containing basic side chains (R, K, and H), and amino acids containing aromatic side chains (H, F, Y, and W) (amino acids are represented by one-letter codes in parenthesis).
  • Amino acid substitutions within each group are called conservative substitutions. It is already known that a polypeptide containing a modified amino acid sequence in which one or more amino acid residues in a given amino acid sequence are deleted, added, and/or substituted with other amino acids can retain the original biological activity ( Mark, D. F. et al., Proc. Natl. Acad. Sci. USA; (1984) 81:5662-6 ; Zoller, M. J. and Smith, M., Nucleic Acids Res. (1982) 10:6487-500 ; Wang, A. et al., Science (1984) 224:1431-3 ; Dalbadie-McFarland, G. et al., Proc. Natl. Acad. Sci.
  • Such mutants have an amino acid identity of at least 70%, more preferably at least 75%, even more preferably at least 80%, still more preferably at least 85%, yet more preferably at least 90%, and most preferably at least 95%, with the variable regions (for example, CDR sequences, FR sequences, or whole variable regions) as disclosed herein.
  • sequence identity is defined as the percentage of residues identical to those in the original amino acid sequence of the heavy chain variable region or light chain variable region, determined after the sequences are aligned and gaps are appropriately introduced to maximize the sequence identity as necessary.
  • sequence identity of amino acid sequences can be determined by the method described below.
  • the amino acid sequences of variable regions that have a substitution, deletion, addition, and/or insertion of one or more amino acids in the amino acid sequence of the variable regions (CDR sequences and/or FR sequences) and retain NR10-binding and/or neutralizing activity can be obtained from nucleic acids that hybridize under stringent conditions to nucleic acid composed of the nucleotide sequence encoding the amino acid sequence of the variable regions.
  • Stringent hybridization conditions to isolate a nucleic acid that hybridizes under stringent conditions to a nucleic acid that includes the nucleotide sequence encoding the amino acid sequence of the variable regions include, for example, the conditions of 6M urea, 0.4% SDS, 0.5x SSC, and 37°C, or hybridization conditions with stringencies equivalent thereto. With more stringent conditions, for example, the conditions of 6M urea, 0.4% SDS, 0.1 x SSC, and 42°C, isolation of nucleic acids with a much higher homology can be expected.
  • the sequences of the isolated nucleic acids can be determined by the known methods described below.
  • the overall nucleotide sequence homology of the isolated nucleic acid is at least 50%, or higher sequence identity, preferably 70% or higher, more preferably 90% .or higher (for example, 95%, 96%, 97%, 98%, 99%, or higher).
  • Nucleic acids that hybridize under stringent conditions to a nucleic acid composed of the nucleotide sequence encoding the amino acid sequence of the variable regions can also be isolated using, instead of the above-described methods using hybridization techniques, gene amplification methods such as polymerase chain reaction (PCR) using primers synthesized based on the information of nucleotide sequence encoding the amino acid sequence of the variable regions.
  • gene amplification methods such as polymerase chain reaction (PCR) using primers synthesized based on the information of nucleotide sequence encoding the amino acid sequence of the variable regions.
  • Whether an antibody recognizes the same epitope as that recognized by another antibody can be confirmed by the competition between the two antibodies against the epitope.
  • Competition between the antibodies can be evaluated by competitive binding assays using means such as ELISA, fluorescence energy transfer method (FRET), and fluorometric microvolume assay technology (FMAT(R)).
  • the amount of antibodies bound to an antigen indirectly correlate with the binding ability of candidate competitor antibodies (test antibodies) that competitively bind to the same epitope. In other words, as the amount of or the affinity of test antibodies against the same epitope increases, the amount of antibodies bound to the antigen decreases, and the amount of test antibodies bound to the antigen increases.
  • appropriately labeled antibodies and antibodies to be evaluated are simultaneously added to the antigens, and the thus bound antibodies are detected using the label.
  • the amount of antibodies bound to the antigen can be easily determined by labeling the antibodies beforehand.
  • This label is not particularly limited, and the labeling method is selected according to the assay technique used.
  • the labeling method includes fluorescent labeling, radiolabeling, enzymatic labeling, and such.
  • fluorescently labeled antibodies and unlabeled antibodies or test antibodies are simultaneously added to animal cells expressing NR10, and the labeled antibodies are detected by fluorometric microvolume assay technology.
  • the "antibody that recognizes the same epitope” refers to an antibody that can reduce the binding of the labeled antibody by at least 50% at a concentration that is usually 100 times higher, preferably 80 times higher, more preferably 50 times higher, even more preferably 30 times higher, and still more preferably 10 times higher than a concentration at which the non-labeled antibody reduces the binding of the labeled antibody by 50% (IC 50 ).
  • Antibodies that bind to the epitope to which the antibodies set forth in any one of (1) to (7) above bind are useful because they have a particularly high neutralizing activity.
  • the antibodies set forth in any one of (1) to (8) above are preferably humanized antibodies, but are not particularly limited thereto.
  • genes encoding the anti-NR10 antibodies of any one of (1) to (8) of (A) to (D) above are disclosed.
  • the genes as disclosed herein may be any form of genes, for example, DNAs or RNAs.
  • Preferred embodiments of the antibodies as disclosed herein include humanized antibodies that bind to NR10.
  • the humanized antibodies can be prepared by methods known to those skilled in the art.
  • variable region of antibody is typically composed of three complementarity-determining regions (CDRs) sandwiched by four frames (FRs).
  • CDRs substantially determine the binding specificity of antibody.
  • the amino acid sequences of CDRs are highly diverse.
  • the amino acid sequences of FRs often exhibit high homology between antibodies having different binding specificities. It is therefore said in general that the binding specificity of an antibody can be transplanted to a different antibody by grafting the CDRs.
  • Humanized antibodies are also referred to as reshaped human antibodies, and they are prepared by transferring the CDRs of an antibody derived from a non-human mammal such as a mouse, to the CDRs of a human antibody.
  • General genetic recombination techniques for their preparation are also known (see European Patent Application Publication No. 125023 and WO 96/02576 ).
  • a DNA sequence designed such that the CDRs of the mouse antibody are linked with framework regions (FRs) of human antibody is synthesized by PCR using, as primers, several oligonucleotides that have portions overlapping the ends of both CDRs and FRs (see the method described in WO 98/13388 ).
  • the resulting DNA is then ligated to a DNA encoding a human antibody constant region, inserted into an expression vector, and introduced into a host to produce the antibody (see European Patent Application Publication No. EP 239400 and International Patent Application Publication No. WO 96/02576 ).
  • Human antibody framework regions to be linked with CDRs are selected so that the CDRs form a favorable antigen-binding site.
  • amino acid substitution, deletion, addition, and/or insertion may be introduced into the framework regions of antibody variable region so that the CDRs of the reshaped human antibody form a proper antigen-binding site.
  • mutations can be introduced into the amino acid sequence of FR by applying the PCR method which is used to graft mouse CDRs to human FRs.
  • mutations can be introduced into a portion of the nucleotide sequences of primers that anneal to the FRs. The mutations are introduced into FRs synthesized by such primers.
  • mutant antibodies having amino acid substitutions can be determined and assessed by the method described above, and thereby mutant FR sequences having desired properties can be selected ( Sato, K. et al., Cancer Res. (1993) 53, 851-856 ).
  • Constant (C) regions from human antibodies are used for those of humanized antibodies.
  • C ⁇ 1, C ⁇ 2, C ⁇ 3, C ⁇ 4, C ⁇ , C ⁇ , C ⁇ 1, C ⁇ 2, and C ⁇ are used for H chains; and C ⁇ and C ⁇ are used for L chains.
  • the amino acid sequence of C ⁇ is shown in SEQ ID NO: 58, and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 57.
  • the amino acid sequence of C ⁇ 1 is shown in SEQ ID NO: 60, and the nucleotide sequence encoding this amino acid sequence is shown in SEQ ID NO: 59.
  • human antibody C regions may be modified to improve the stability of antibody or antibody production. Modified human antibody C regions include, for example, the C regions described herein below.
  • Human antibodies used for humanization may be of any isotype such as IgG, IgM, IgA, IgE, or IgD; however, IgG is preferably used in the present invention. IgG that can be used includes IgG1, IgG2, IgG3, IgG4, and the like.
  • amino acids in the variable region for example, CDR and FR
  • constant region of the humanized antibody may be deleted, added, inserted, and/or substituted with other amino acids.
  • the antibodies as disclosed herein also include such humanized antibodies with amino acid substitutions and the like.
  • the origin of CDRs of a humanized antibody is not particularly limited, and may be any animal.
  • Humanized antibodies are useful when administered to humans for the therapeutic purposes, because they exhibit reduced immunogenicity in the human body.
  • humanized anti-NR10 antibodies as disclosed herein include, for example:
  • the heavy chain variable region having the amino acid sequence of SEQ ID NO: 50 (H0-VH), heavy chain variable region having the amino acid sequence of SEQ ID NO: 112, and light chain variable region having the amino acid sequence of SEQ ID NO: 52 (L0-VL) may have a substitution, deletion, addition, and/or insertion of one or more amino acids.
  • the substitution, deletion, addition, and/or insertion of amino acids may be made in either or both of the CDRs and FRs.
  • humanized anti-NR10 antibody as disclosed herein include, for example:
  • the antibodies of any one of (f) to (j) preferably have an activity similar to that of the antibodies of any one of (a) to (e).
  • substitution, deletion, addition, and/or insertion of amino acids are not particularly limited, but specific examples include, for example, the above-described amino acid substitutions.
  • amino acid substitutions may be included:
  • substitutions other than those described above include a substitution of Arg at position 3 of heavy chain FR2 having the amino acid sequence of SEQ ID NO: 97 with another amino acid.
  • the amino acid after substitution is not particularly limited; but preferred examples thereof include Gin.
  • Arg at position 3 in SEQ ID NO: 97 has been replaced with Gln
  • Ala at position 5 may be substituted with Ser to produce a human FR2 sequence.
  • the amino acid sequence in which Arg and Ala at positions 3 and 5 in the amino acid sequence of SEQ ID NO: 97 have been replaced with Gln and Ser, respectively, is shown in SEQ ID NO: 120.
  • the present invention provides heavy chain variable regions in which FR2 having the amino acid sequence of SEQ ID NO: 97 is substituted with FR2 having the amino acid sequence of SEQ ID NO: 120 in a heavy chain variable region having the amino acid sequence of SEQ ID NO: 50 or 112.
  • amino acid substitutions may be used alone or in combination with other amino acid substitutions described above. They also may be combined with amino acid substitutions other than those described above.
  • antibodies in which the above-described substitutions have been carried out include, for example, antibodies that comprise a heavy chain variable region having the amino acid sequence of SEQ ID NO: 167, antibodies that comprise a light chain variable region having the amino acid sequence of SEQ ID NO: 168, and antibodies that comprise a heavy chain variable region having the amino acid sequence of SEQ ID NO: 167 and a light chain variable region having the amino acid sequence of SEQ ID NO: 168.
  • heavy chain variable regions in which the above-described substitutions have been carried out include, for example, the following heavy chain variable regions:
  • antibodies comprising the above-described heavy chain and light chain variable regions include, for example, the following antibodies:
  • the constant region used for the humanized antibodies as disclosed herein may be any constant region derived from a human antibody.
  • Preferred examples of such constant regions derived from human antibodies include, for example, constant regions derived from IgG1 or IgG2.
  • constant regions in which one or more amino acids are substituted, deleted, added, and/or inserted in the constant region derived from a human antibody may also be used.
  • constant regions in which one or more amino acids are substituted, deleted, added, and/or inserted in.the constant region derived from a human antibody are not particularly limited, and include, for example, the following constant regions:
  • heavy chains or antibodies having the above-described constant regions include, for example:
  • humanized anti-NR10 antibodies as disclosed herein include, for example, the following antibodies:
  • the heavy chain having the amino acid sequence of SEQ ID NO: 54 (H0-VH + constant region) and the light chain having the amino acid sequence of SEQ ID NO: 56 (L0-VL + constant region) may have a substitution, deletion, addition, and/or insertion of one or more amino acids.
  • the substitution, deletion, addition, and/or insertion of amino acids may be carried out in either or both of the variable and constant regions.
  • the antibodies of any one of (p) to (t) preferably have an activity similar to that of the antibodies of any one of (k) to (o).
  • substitution, deletion, addition, and/or insertion of amino acids are not particularly limited, but specific examples thereof include, for example, the above-described amino acid substitutions.
  • nucleotide sequence encoding the amino acid sequence of the above-described humanized heavy chain variable region is shown in SEQ ID NO: 49.
  • the nucleotide sequence encoding the amino acid sequence of the humanized light chain variable region is shown in SEQ ID NO: 51.
  • the nucleotide sequence encoding the amino acid sequence of the humanized heavy chain is shown in SEQ ID NO: 54.
  • the nucleotide sequence encoding the amino acid sequence of the humanized light chain (SEQ ID NO: 56) is shown in SEQ ID NO: 55.
  • the present invention provides the following heavy and light chains and antibodies:
  • substitution, deletion, addition, and/or insertion of amino acids are as described above.
  • Antibodies that recognize the same epitope as recognized by an antibody are also described above.
  • variable regions genes encoding the variable regions, heavy chains, light chains, or antibodies of the present invention.
  • variable regions, heavy chains, light chains, or antibodies of the present invention which comprise the step of culturing the above-described host cells.
  • the vectors, host cells, and culture of host cells are described herein below.
  • domain 1 refers to the region of amino acids at positions 21 to 120 (LPAKP to LENIA) in the amino acid sequence of human NR10 of SEQ ID NO: 76, where the amino acid numbering is based on the sequence including the signal peptide.
  • domain 2 refers to the region of amino acids at positions 121 to 227 (KTEPP to EEEAP) in the amino acid sequence of human NR10 of SEQ ID NO: 76, where the amino acid numbering is based on the sequence including the signal peptide.
  • Such antibodies are not particularly limited; however, in general, they have a neutralizing activity, and preferably are humanized antibodies.
  • Examples of the preferred antibodies as disclosed herein include antibodies that recognize domain 1.
  • the antibodies that recognize domain 1 have a strong neutralizing activity, and thus are particularly useful as pharmaceuticals.
  • Antibodies neutralizing activity
  • anti-NR10 antibodies having a neutralizing activity.
  • the neutralizing activity against NR10 refers to an activity of inhibiting the binding between NR10 and its ligand IL-31, and preferably an activity of suppressing a biological activity based on NR10.
  • Antibodies having a NR10-neutralizing activity can be selected, for example, by adding candidate antibodies to an IL-31-dependent cell line and observing their growth-suppressing effect on the cell line. In this method, antibodies that suppress the growth of the IL-31-dependent cell line are determined as antibodies having a neutralizing activity against NR10.
  • the antibodies as disclosed herein are not limited in terms of their origin, and may be derived from any animals such as humans, mice, and rats. Moreover, the antibodies may be recombinant antibodies such as chimeric antibodies and humanized-antibodies. As described above, the preferred antibodies as disclosed herein include humanized antibodies.
  • the chimeric antibodies contain, for example, the heavy and light chain constant regions of a human antibody, and the heavy and light chain variable regions of an antibody of a non-human mammal, such as mouse.
  • the chimeric antibodies can be produced by known methods.
  • the antibodies can be produced by cloning an antibody gene from hybridomas, inserting it into an appropriate vector, and introducing the construct into hosts (see, for example, Carl, A. K. Borrebaeck, James, W. Larrick, THERAPEUTIC MONOCLONAL ANTIBODIES, Published in the United Kingdom by MACMILLAN PUBLISHERS LTD, 1990 ).
  • V regions cDNAs of the antibody variable regions (V regions) are synthesized from mRNA of hybridomas using reverse transcriptase. Once DNAs encoding the V regions of an antibody of interest are obtained, these are linked witch DNAs encoding the constant regions (C regions) of a desired human antibody. The resulting constructs are inserted into expression vectors.
  • the DNAs encoding the antibody V regions may be inserted into expression vectors comprising DNAs encoding the C regions of a human antibody.
  • the DNAs are inserted into expression vectors so that they are expressed under the regulation of the expression regulatory regions, for example, enhancers and promoters.
  • host cells can be transformed with the expression vectors to allow expression of chimeric antibodies.
  • desired human antibodies with antigen-binding activity can be obtained by (1) sensitizing human lymphocytes with antigens of interest or cells expressing antigens of interest in vitro; and (2) fusing the sensitized lymphocytes with human myeloma cells such as U266 (see Japanese Patent Application Kokoku Publication No. (JP-B) H01-59878 (examined, approved Japanese patent application published for opposition)).
  • the desired human antibody can also be obtained by immunizing a transgenic animal having an entire repertoire of human antibody genes with a desired antigen (see International Patent Application Publication Nos. WO 93/12227 , WO 92/03918 , WO 94/02602 , WO 94/25585 , WO 96/34096 , and WO 96/33735 ).
  • variable region of a human antibody is expressed as a single chain antibody (scFv) on the surface of a phage, using a phage display method, and phages that bind to the antigen can be selected.
  • scFv single chain antibody
  • the DNA sequences encoding the variable regions of human antibodies that bind to the antigen can be determined. If the DNA sequences of scFvs that bind to the antigen are identified, appropriate expression vectors comprising these sequences can be constructed to obtain human antibodies. Such methods are well known.
  • the antibodies as disclosed herein include not only divalent antibodies as represented by IgG, but also monovalent antibodies, multivalent antibodies as represented by IgM, and bispecific antibodies capable of binding to different antigens, as long as they have a NR10-binding activity and/or neutralizing activity.
  • the multivalent antibodies as disclosed herein include multivalent antibodies in which the antigen-binding sites are all identical, and multivalent antibodies in which all or some of the antigen-binding sites are different.
  • the antibodies as disclosed herein are not limited to full-length antibody molecules, but may also be low-molecular-weight antibodies or modified products thereof, as long as they bind to NR10 protein.
  • the antibodies as disclosed herein may be low-molecular-weight antibodies.
  • Such low-molecular-weight antibodies are antibodies including antibody fragments lacking some portions of a whole antibody (for example, whole IgG), and are not particularly limited as long as they retain NR10-binding and/or neutralizing activity.
  • the low-molecular-weight antibodies are not particularly limited, as long as they contain a portion of whole antibodies.
  • the low-molecular-weight antibodies preferably contain a heavy chain variable region (VH) or light chain variable region (VL). Particularly preferred low-molecular-weight antibodies contain both VH and VL.
  • low-molecular-weight antibodies of the present invention include low-molecular-weight antibodies containing CDRs of an antibody.
  • the CDRs contained in the low-molecular-weight antibodies may include some or all of the six CDRs of an antibody.
  • the low-molecular-weiglit antibodies as disclosed herein preferably have a smaller molecular weight than whole antibodies.
  • the low-molecular-weight antibodies may form multimers, for example, dimers, trimers, or tetramers, and thus their molecular weights can be greater than those of whole antibodies.
  • antibody fragments include, for example, Fab, Fab', F(ab')2, and Fv.
  • specific examples of the low-molecular-weight antibodies include, for example, Fab, Fab', F(ab')2, Fv, scFv (single chain Fv), diabodies, and sc(Fv)2 (single chain (Fv)2).
  • Multimers for example, dimers, trimers, tetramers, and polymers
  • these antibodies are also included in the low-molecular-weight antibodies as disclosed herein.
  • Antibody fragments can be obtained, for example, by treating antibodies with enzymes to produce antibody fragments.
  • Enzymes known to generate antibody fragments include, for example, papain, pepsin, and plasmin.
  • a gene encoding such an antibody fragment can be constructed, introduced into an expression vector, and expressed in appropriate host cells (see, for example, Co, M.S. et al., J. Immunol. (1994)152, 2968-2976 ; Better, M. & Horwitz, A. H. Methods in Enzymology (1989)178, 476-496 ; Plueckthun, A. & Skerra, A.
  • Digestive enzymes cleave a specific site of an antibody fragment, yielding antibody fragments of specific structures shown below. Genetic engineering techniques can be applied to such enzymatically-obtained antibody fragments to delete an arbitrary portion of the antibody.
  • Antibody fragments obtained by using the above-described digestive enzymes are as follows:
  • the low-molecular-weight antibodies as disclosed herein include antibody fragments lacking an arbitrary region, as long as they have a NR10-binding activity and/or neutralizing activity.
  • Diabodies refers to a bivalent antibody fragment constructed by gene fusion ( Holliger P et al., Proc. Natl. Acad. Sci. USA 90: 6444-6448 (1993 ); EP 404,097 ; WO 93/11161 , etc).
  • Diabodies are dimers composed of two polypeptide chains. In each of the polypeptide chains forming a dimer, a VL and a VH are usually linked by a linker in the same chain.
  • the linker in a diabody is short enough such that the VL and VH cannot bind to each other.
  • the number of amino acid residues constituting the linker is, for example, about five residues.
  • the VL and VH encoded on the same polypeptide cannot form a single-chain variable region fragment, and will form a dimer with another single-chain variable region fragment.
  • the diabody has two antigen binding sites.
  • ScFv antibodies are single-chain polypeptides produced by linking a heavy chain variable region ([VH]) and a light chain variable region ([VL]) via a linker or such ( Huston, J. S. et al., Proc. Natl. Acad. Sci. U.S.A. (1988) 85, 5879-5883 ; Pluckthun "The Pharmacology of Monoclonal Antibodies” Vol. 113, eds., Resenburg and Moore, Springer Verlag, New York, pp. 269-315, (1994 )).
  • the H-chain V region and L-chain V region of scFv may be derived from any antibody described herein.
  • the peptide linker for linking the V regions is not particularly limited. For example, an arbitrary single-chain peptide containing about three to 25 residues can be used as the linker. Specifically, it is possible to use the peptide linkers or such described below.
  • V regions of both chains can be linked, for example, by PCR as described above.
  • PCR a DNA encoding a complete or desired partial amino acid sequence is used as a template to link the V regions by PCR:
  • DNAs encoding the V regions of H chain and L chain are amplified by PCR using a pair of primers having sequences corresponding to those at both ends of the DNA to be amplified. Then, a DNA encoding the peptide linker portion is prepared.
  • the peptide linker-encoding DNA can also be synthesized by PCR. Here, nucleotide sequences that can be ligated to the amplification products of V regions synthesized separately are added to the 5' end of the primers to be used. Then, PCR is carried out using each DNA of the [H chain V region DNA] [peptide linker DNA] - [L chain V region DNA], and assembly PCR primers.
  • the assembly PCR primers are composed of a combination of a primer that anneals to the 5' end of the [H chain V region DNA] and a primer that anneals to the 3' end of the [L chain V region DNA].
  • the assembly PCR primers are a set of primers that can be used to amplify DNA encoding the full-length sequence of scFv to be synthesized.
  • nucleotide sequences that can be ligated to the V-region DNAs have been added to the [peptide linker DNA].
  • these DNAs are linked together, and then the whole scFv is ultimately generated as an amplification product by the assembly PCR primers.
  • expression vectors carrying these DNAs and recombinant cells transformed with these expression vectors can be obtained by conventional methods. Furthermore, the scFv can be obtained by culturing the resulting recombinant cells to express the scFv-encoding DNAs.
  • the order of the heavy chain and light chain variable regions to be linked together is not particularly limited, and they may be arranged in any order. Examples of the arrangement are listed below.
  • sc(Fv)2 is a single-chain low-molecular-weight antibody produced by linking two VHs and two VLs using linkers and such ( Hudson et al., J Immunol. Methods 1999 ; 231: 177-189 ).
  • sc(Fv)2 can be produced by linking scFvs via a linker.
  • Antibodies in which two VHs and two VLs are arranged in the order of VH-VL-VH-VL ([VH] linker [VL] linker [VH] linker [VL]) from the N terminus of the single-chain polypeptide are preferred.
  • the order of the two VHs and two VLs is not limited to the above arrangement, and they may be arranged in any order. Examples of the arrangement are listed below:
  • the amino acid sequence of the heavy chain variable region or light chain variable region in a low-molecular-weight antibody may contain a substitution, deletion, addition, and/or insertion.
  • the heavy chain variable region and light chain variable region may also lack some portions or be added with other polypeptides, as long as they have antigen binding ability when linked together.
  • the variable regions may be chimerized or humanized.
  • linkers which bind the variable regions of the antibody include arbitrary peptide linkers that can be introduced using genetic engineering, or synthetic linkers such as those disclosed in Protein Engineering, 9(3), 299-305, 1996 .
  • the preferred linkers are peptide linkers.
  • the lengths of the peptide linkers are not particularly limited and those skilled in the art can appropriately select the lengths depending on the purpose. Typical lengths are one to 100 amino acids, preferably 3 to 50 amino acids, more preferably 5 to 30 amino acids, and particularly preferably 12 to 18 amino acids (for example, 15 amino acids).
  • amino acid sequences of such peptide linkers include, for example:
  • amino acid sequence of peptide linker can be appropriately selected by those skilled in the art depending on the purpose.
  • n which determines the length of the peptide linker, is usually 1 to 5, preferably 1 to 3, and more preferably 1 or 2.
  • Synthetic linkers include crosslinking-agents that are routinely used to crosslink peptides, for example, N-hydroxy succinimide (NHS), disuccinimidyl suberate (DSS), bis(sulfosuccinimidyl) suberate (BS 3 ), dithiobis(succinimidyl propionate) (DSP), dithiobis(sulfosuccinimidyl propionate) (DTSSP), ethylene glycol bis(succinimidyl succinate) (EGS), ethylene glycol bis(sulfosuccinimidyl succinate) (sulfo-EGS), disuccinimidyl tartrate (DST), disulfosuccinimidyl tartrate (sulfo-DST), bis[2-(succinimidoxycarbonyloxy)ethyl] sulfone (BSOCOES), and bis[2-(sulfosuccinimide
  • linkers When four antibody variable regions are linked, three linkers are usually required. Such multiple linkers may be the same or different.
  • the antibodies as disclosed herein include antibodies in which one or more amino acid residues have been added to the amino acid sequence of an antibody of the present invention.
  • fusion proteins which result from a fusion between one of the above antibodies and a second peptide or protein is included in the present invention.
  • the fusion proteins can be prepared by ligating a polynucleotide encoding an antibody as disclosed herein and a polynucleotide encoding a second peptide or polypeptide in frame, inserting this into an expression vector, and expressing the fusion construct in a host.
  • the partner peptide or polypeptide to be fused with an antibody of the present invention may be a known peptide, for example, FLAG ( Hopp, T. P. et al., BioTechnology 6, 1204-1210 (1988 )), 6x His consisting of six His (histidine) residues, 10x His, influenza hemagglutinin (HA), human c-myc fragment, VSV-GP fragment, p18HIV fragment, T7-tag, HSV-tag, E-tag, SV40 T antigen fragment, lck tag, ⁇ -tubulin fragment, B-tag, Protein C fragment.
  • FLAG Hopp, T. P. et al., BioTechnology 6, 1204-1210 (1988 )
  • 6x His consisting of six His (histidine) residues, 10x His, influenza hemagglutinin (HA), human c-myc fragment, VSV-GP fragment, p18HIV fragment, T7-tag, HSV-tag, E-tag
  • partner polypeptides to be fused with the antibodies of the present invention include, for example, GST (glutathione-S-transferase), HA (influenza hemagglutinin), immunoglobulin constant region, ⁇ -galactosidase, and MBP (maltose-binding protein).
  • GST glutthione-S-transferase
  • HA influenza hemagglutinin
  • immunoglobulin constant region e.gly available peptides or polypeptides
  • ⁇ -galactosidase ⁇ -galactosidase
  • MBP maltose-binding protein
  • the antibodies as disclosed herein may be conjugated antibodies which are linked to any of various molecules including polymeric substances such as polyethylene glycol (PEG) and hyaluronic acid, radioactive substances, fluorescent substances, luminescent substances, enzymes, and toxins.
  • conjugated antibodies can be obtained by chemically modifying the obtained antibodies. Methods for modifying antibodies have been established in this field (for example, US 5057313 and US 5156840 ).
  • the "antibodies" of the present invention also include such conjugated antibodies.
  • the antibodies used in the present disclosure may be bispecific antibodies.
  • the bispecific antibody refers to an antibody that has variable regions recognizing different epitopes in the same antibody molecule.
  • the bispecific antibodies may recognize different epitopes on an NR10 molecule, or recognize NR10 with one antigen-binding site and a different substance with the other antigen-binding site.
  • Bispecific antibodies can be prepared, for example, by linking two antibodies that recognize different antigens. Antibodies to be linked together may be half molecules each of which contains an H chain and an L chain, or quarter molecules that consist of only one H chain. Alternatively, hybridomas producing different monoclonal antibodies can be fused to produce a bispecific antibody-producing fused cell. Furthermore, bispecific antibodies can be produced by genetic engineering techniques.
  • the antibodies as disclosed herein may differ in amino acid sequence, molecular weight, isoelectric point, presence/absence of sugar chains, and conformation depending on the cell or host producing the antibody or the purification method as described below.
  • a resulting antibody is included in the present disclosure, as long as it is functionally equivalent to an antibody of the present invention.
  • an antibody of the present invention when expressed in prokaryotic cells, for example E. coli, a methionine residue is added to the N terminus of the original antibody amino acid sequence.
  • Such antibodies are included in the present disclosure.
  • the antibodies as disclosed herein may be polyclonal or monoclonal antibodies.
  • Such monoclonal antibodies having NR10-binding and/or neutralizing activity can be obtained, for example, by the following procedure: anti-NR10 monoclonal antibodies are prepared by using as an antigen NR10 or a fragment thereof that is derived from a mammal such as human or mouse by known methods, and then antibodies having NR10-binding and/or neutralizing activity are selected from the thus obtained anti-NR10 monoclonal antibodies.
  • a desired antigen or cells expressing the desired antigen are used as a sensitizing antigen for immunization according to conventional immunization methods.
  • Anti-NR10 monoclonal antibodies can be prepared by fusing the obtained immune cells with known parental cells using conventional cell fusion methods, and screening them for monoclonal antibody-producing cells (hybridomas) by conventional screening methods.
  • Animals to be immunized include, for example, mammals such as mice, rats, rabbits, sheep, monkeys, goats, donkeys, cows, horses, and pigs.
  • the antigen can be prepared using the known NR10 gene sequence according to known methods, for example, by methods using baculovirus (for example, WO 98/46777 ).
  • Hybridomas can be prepared, for example, according to the method of Milstein et al. ( Kohler, G. and Milstein, C., Methods Enzymol. (1981) 73: 3-46 ) or such.
  • immunization may be performed after linking the antigen with a macromolecule having immunogenicity, such as albumin.
  • Embodiments of the antibodies as disclosed herein that have a binding and/or neutralizing activity against NR10 include monoclonal antibodies that have a binding and/or neutralizing activity against human NR10.
  • Antigens used to prepare monoclonal antibodies, that have a binding and/or neutralizing activity against human NR10 are not particularly limited, as long as they enable preparation of antibodies that have a binding and/or neutralizing activity against human NR10.
  • Human NR10.3 is one of preferred immunogens in preparing antibodies that have an activity of binding and/or neutralizing NR10 in the present invention.
  • the binding and/or neutralizing activity of antibody against NR10 can be measured, for example, by observing the effect of suppressing the growth of the IL-31-dependent cell line as described in the Examples.
  • DNA immunization is a method in which a vector DNA constructed such that the gene encoding an antigen protein can be expressed in an animal to be immunized is administered to the animal, and the immunogen is expressed within the body of the animal to provide immunostimulation.
  • the DNA immunization is expected to be advantageous in that:
  • DNA encoding NR10 is administered to an animal to be immunized.
  • the DNA encoding NR10 can be synthesized by known methods such as PCR.
  • the resulting DNA is inserted into an appropriate expression vector, and administered to the animal to be immunized.
  • Expression vectors that can be used include commercially available expression vectors such as pcDNA3.1.
  • the vector can be administered to the living body by conventional methods.
  • DNA immunization can be carried out by introducing gold particles coated with the expression vector into cells by gene gun.
  • Booster using NR10-expressing cells after DNA immunization is a preferred method to yield a monoclonal antibody.
  • immune cells are collected from the mammal and subjected to cell fusion.
  • Preferred immune cells are spleen cells in particular.
  • Mammalian myeloma cells are used for fusion with the above immune cells. It is preferred that myeloma cells have appropriate selection markers for screening.
  • the selection marker refers to a phenotype that allows (or does not allow) survival under particular culture conditions.
  • Known selection markers include hypoxanthine-guanine phosphoribosyltransferase deficiency (hereinafter abbreviated as "HGPRT deficiency”) and thymidine kinase deficiency (hereinafter abbreviated as "TK deficiency”).
  • HGPRT- or TK-deficient cells exhibit hypoxanthine-aminopterin-thymidine sensitivity (hereinafter abbreviated as "HAT sensitivity”).
  • HAT selection medium HAT-sensitive cells cannot synthesize DNA and thus will die. However, when fused with normal cells, they can continue to synthesize DNA via the salvage pathway of the normal cells and thus can grow even in HAT selection medium.
  • HGPRT- or TK-deficient cells can be selected using a medium containing 6-thioguanine, 8-azaguanine (hereinafter abbreviated as "8AG"), or 5'-bromodeoxyuridine. While normal cells are killed due to incorporation of these pyrimidine analogs into DNA, cells lacking these enzymes can survive in the selection medium because they cannot incorporate these pyrimidine analogs.
  • Another selection marker called G418 resistance confers resistance to 2-deoxystreptamine antibiotics (gentamicin analogs) due to the neomycin resistance gene.
  • gentamicin analogs due to the neomycin resistance gene.
  • myeloma cells suitable for cell fusion are known.
  • Cell fusion between immune cells and myeloma cells can be essentially carried out according to known methods, for example, the method by Kohler and Milstein ( Kohler. G. and Milstein, C., Methods Enzymol. (1981) 73, 3-46 ).
  • cell fusion can be carried out, for example, in a common culture medium in the presence of a cell fusion-promoting agent.
  • the fusion-promoting agent includes, for example, polyethylene glycol (PEG) and Sendai virus (HVJ).
  • PEG polyethylene glycol
  • HVJ Sendai virus
  • an auxiliary agent such as dimethyl sulfoxide may also be added to improve fusion efficiency.
  • the immune cells and myeloma cells may be used at an arbitrarily determined ratio.
  • the ratio of immune cells to myeloma cells is preferably from 1 to 10.
  • Culture media to be used for cell fusion include, for example, media that are suitable for the cell growth of myeloma cell line, such as RPMI 1640 and MEM, and other common culture media used for this type of cell culture.
  • the culture media may also be supplemented with serum supplement such as fetal calf serum (FCS).
  • FCS fetal calf serum
  • Predetermined amounts of immune cells and myeloma cells are mixed well in the culture medium, and then mixed with a PEG solution pre-heated to 37°C to produce fused cells (hybridomas).
  • a PEG solution pre-heated to 37°C pre-heated to 37°C
  • fused cells fused cells
  • PEG with mean molecular weight of about 1,000-6,000 can be added to the cells typically at a concentration of 30% to 60% (w/v).
  • successive addition of the appropriate culture medium listed above and removal of supernatant by centrifugation are repeated to eliminate the cell fusion agent and such, which are unfavorable to the growth of hybridomas.
  • the resulting hybridomas can be screened using a selection medium according to the selection marker possessed by myeloma cells used in the cell fusion.
  • a selection medium a medium containing hypoxanthine, aminopterin, and thymidine.
  • HAT medium a medium containing hypoxanthine, aminopterin, and thymidine.
  • the desired hybridomas can be selected by culturing the cells for several days to several weeks. Then, screening and single cloning of hybridomas that produce an antibody of interest can be carried out by performing ordinary limiting dilution methods.
  • antibodies that recognize NR10 can be prepared by the method described in WO 03/104453 .
  • an antigen is bound to a carrier such as beads made of polystyrene or such and commercially available 96-well microtiter plates, and then reacted with the culture supernatant of hybridoma.
  • a carrier such as beads made of polystyrene or such and commercially available 96-well microtiter plates, and then reacted with the culture supernatant of hybridoma.
  • the carrier is washed and then reacted with an enzyme-labeled secondary antibody or such.
  • the culture supernatant contains an antibody of interest reactive to the sensitizing antigen
  • the secondary antibody binds to the carrier via this antibody.
  • the secondary antibody bound to the carrier is detected to determine whether the culture supernatant contains the antibody of interest.
  • Hybridomas producing a desired antibody capable of binding to the antigen can be cloned by the limiting dilution method or such.
  • an antigen used for immunization but also an NR10 protein substantially equivalent thereto can be preferably used as an antigen for this purpose.
  • a cell line expressing NR10, the extracellular domain of NR10, or an oligopeptide composed of a partial amino acid sequence constituting the domain may be used as the antigen.
  • antibodies of interest can also be obtained by sensitizing human lymphocytes with an antigen. Specifically, first, human lymphocytes are sensitized with an NR10 protein in vitro . Then, the sensitized lymphocytes are fused with an appropriate fusion partner. For example, human-derived myeloma cells with the ability to divide permanently can be used as the fusion partner (see Japanese Patent Application Kokoku Publication No. (JP-B) H1-59878 (examined, approved Japanese patent application published for opposition). Antibodies obtained by this method are human antibodies having an activity of binding to the NR10 protein.
  • nucleotide sequence encoding an anti-NR10 antibody obtained by the above-described method or such, and its amino acid sequence can be obtained by methods known to those skilled in the art.
  • Amino acids contained in the amino acid sequences described in the present invention may undergo post-translational modification (for example, modification of N-terminal glutamine into pyroglutamic acid by pyroglutamylation is well-known to persons skilled in the art).
  • post-translational modification for example, modification of N-terminal glutamine into pyroglutamic acid by pyroglutamylation is well-known to persons skilled in the art.
  • sequences with post-translationally modified amino acids are also included in the amino acid sequences described in the present invention.
  • the anti-NR10 antibody can be prepared, for example, by genetic recombination techniques known to those skilled in the art. Specifically, a polynucleotide encoding an antibody can be constructed based on the sequence of the NR10-recognizing antibody, inserted into an expression vector, and then expressed in appropriate host cells (see for example, Co, M. S. et al., J. Immunol. (1994) 152, 2968-2976 ; Better, M. and Horwitz, A. H., Methods Enzymol. (1989) 178, 476-496 ; Pluckthun, A. and Skerra, A., Methods Enzymol.
  • the vectors include M13 vectors, pUC vectors, pBR322, pBluescript, and pCR-Script.
  • the vectors include, for example, pGEM-T, pDIRECT, and pT7, in addition to the vectors described above.
  • Expression vectors are particularly useful when using vectors for producing the antibodies of the present invention. For example, when aiming for expression in E. coli such as JM109, DH5 ⁇ , HB101, and XL1-Blue, the expression vectors not only have the above-described characteristics that allow vector amplification in E. coli, but must also carry a promoter that allows efficient expression in E.
  • coli for example, lacZ promoter ( Ward et al., Nature (1989) 341, 544-546 ; FASEB J. (1992) 6, 2422-2427 ), araB promoter ( Better et al., Science (1988) 240, 1041-1043 ), T7 promoter or such.
  • lacZ promoter Ward et al., Nature (1989) 341, 544-546 ; FASEB J. (1992) 6, 2422-2427
  • araB promoter Better et al., Science (1988) 240, 1041-1043
  • T7 promoter or such Such vectors include pGEX-5X-1 (Pharmacia), "QIAexpress system” (Qiagen), pEGFP, or pET (in this case, the host is preferably BL21 that expresses T7 RNA polymerase) in addition to the vectors described above.
  • the vectors may contain signal sequences for antibody secretion.
  • a signal sequence for antibody secretion a pelB signal sequence ( Lei, S. P. et al J. Bacteriol. (1987) 169, 4379 ) may be used when a protein is secreted into the E. coli periplasm.
  • the vector can be introduced into host cells by calcium chloride or electroporation methods, for example.
  • the vectors for producing the antibodies of the present invention include mammalian expression vectors (for example, pcDNA3 (Invitrogen), pEF-BOS ( Nucleic Acids. Res. 1990, 18(17), p5322 ), pEF, and pCDM8), insect cell-derived expression vectors (for example, the "Bac-to-BAC baculovirus expression system" (Gibco-BRL) and pBacPAK8), plant-derived expression vectors (for example, pMH1 and pMH2), animal virus-derived expression vectors (for example, pHSV, pMV, and pAdexLcw), retroviral expression vectors (for example, pZIPneo), yeast expression vectors (for example, "Pichia Expression Kit” (Invitrogen), pNV11, and SP-Q01), and Bacillus subtilis expression vectors (for example, pPL608 and pKTH50), for example, pcDNA3 (Invit
  • the vectors When aiming for expression in animal cells such as CHO, COS, and NIH3T3 cells, the vectors must have a promoter essential for expression in cells, for example, SV40 promoter ( Mulligan et al., Nature (1979) 277, 108 ), MMLV-LTR promoter; EF1 ⁇ promoter ( Mizushima et al., Nucleic Acids Res. (1990) 18, 5322 ), and CMV promoter, and more preferably they have a gene for selecting transformed cells (for example, a drug resistance gene that allows evaluation using an agent (neomycin, G418, or such).
  • Vectors with such characteristics include pMAM, pDR2, pBK-RSV, pBK-CMV, pOPRSV, and pOP13, for example.
  • the following method can be used for stable gene expression and gene amplification in cells: CHO cells deficient in a nucleic acid synthesis pathway are introduced with a vector (for example, pSV2-dhfr ( Molecular Cloning 2nd edition, Cold Spring Harbor Laboratory Press, 1989 )) that carries a DHFR gene which compensates for the deficiency, and the vector is amplified using methotrexate (MTX).
  • a vector for example, pSV2-dhfr ( Molecular Cloning 2nd edition, Cold Spring Harbor Laboratory Press, 1989 )
  • MTX methotrexate
  • the following method can be used for transient gene expression: COS cells with a gene expressing SV40 T antigen on their chromosome are transformed with a vector (pcD and such) with an SV40 replication origin.
  • Replication origins derived from polyoma virus, adenovirus, bovine papilloma virus (BPV), and such can also be used.
  • the expression vectors may further carry selection markers such as aminoglycoside transferase (APH) gene, thymidine kinase (TK) gene, E. coli xanthine-guanine phosphoribosyltransferase (Ecogpt) gene, and dihydrofolate reductase (dhfr) gene.
  • APH aminoglycoside transferase
  • TK thymidine kinase
  • Ecogpt E. coli xanthine-guanine phosphoribosyltransferase
  • dhfr dihydrofolate reductase
  • the antibodies as disclosed herein obtained by the methods described above can be isolated from inside host cells or from outside the cells (the medium, or such), and purified to homogeneity.
  • the antibodies can be isolated and purified by methods routinely used for isolating and purifying antibodies, and the type of method is not limited.
  • the antibodies can be isolated and purified by appropriately selecting and combining column chromatography, filtration, ultrafiltration, salting out, solvent precipitation, solvent extraction, distillation, immunoprecipitation, SDS-polyacrylamide gel electrophoresis, isoelectrofocusing, dialysis, recrystallization, and such.
  • the chromatographies include, for example, affinity chromatography, ion exchange chromatography, hydrophobic chromatography, gel filtration, reverse phase chromatography, and adsorption chromatography ( strategies for Protein Purification and Characterization: A Laboratory Course Manual. Ed Daniel R. Marshak et al., Cold Spring Harbor Laboratory Press, 1996 ).
  • the chromatographic methods described above can be conducted using liquid chromatography, for example, HPLC and FPLC.
  • Columns that can be used for affinity chromatography include protein A columns and protein G columns.
  • Columns using protein A include, for example, Hyper D, POROS, and Sepharose FF (GE Amersham Biosciences). There are disclosed antibodies that are highly purified using these purification methods.
  • the NR10-binding activity of the obtained antibodies can be determined by methods known to those skilled in the art.
  • Methods for determining the antigen-binding activity of an antibody include, for example, ELISA (enzyme-linked immunosorbent assay), EIA (enzyme immunoassay), RIA (radioimmunoassay), and fluorescent antibody method.
  • enzyme immunoassay enzyme immunoassay
  • antibody-containing samples such as purified antibodies and culture supernatants of antibody-producing cells, are added to antigen-coated plates.
  • a secondary antibody labeled with an enzyme, such as alkaline phosphatase is added and the plates are incubated. After washing, an enzyme substrate, such as p-nitrophenyl phosphate, is added, and the absorbance is measured to evaluate the antigen-binding activity.
  • the present invention also provides pharmaceutical compositions comprising the antibody mentioned above as an active ingredient. Moreover, the present invention provides therapeutic agents for inflammatory diseases which comprise the antibody mentioned above as an active ingredient.
  • inflammatory disease refers to diseases with pathological features involved in cytological and histological reactions that occur in affected blood vessels and adjacent tissues in response to an injury or abnormal stimulation caused by physical, chemical, or biological agents ( Stedman's Medical Dictionary, 5th Ed., MEDICAL VIEW CO., 2005 ).
  • inflammatory diseases include, dermatitis (atopic dermatitis, chronic dermatitis, and such), inflammatory bowel diseases (colitis and such), asthma, arthritis (rheumatoid arthritis, osteoarthritis, and such), bronchitis, Th2 autoimmune diseases, systemic lupus erythematosus, myasthenia gravis, chronic GVHD, Crohn's disease, spondylitis deformans, lumbar pain, gout, inflammation after surgery or injury, swelling, neuralgia, laryngopharyngitis, cystitis, hepatitis (non-alcoholic steatohepatitis, alcoholic hepatitis, and such), hepatitis B, hepatitis C, arteriosclerosis, and pruritus.
  • dermatitis atopic dermatitis, chronic dermatitis, and such
  • inflammatory bowel diseases colitis and such
  • asthma arthritis
  • arthritis rheumatoid arthritis, osteoarth
  • Preferred examples of inflammatory diseases that are subjects of the present invention include atopic dermatitis, chronic dermatitis, rheumatism, osteoarthritis, chronic asthma, and pruritus.
  • an anti-NR10 antibody as an active ingredient means comprising an anti-NR10 antibody as at least one of the active ingredients, and does not limit the proportion of the antibody.
  • the therapeutic agents for inflammatory diseases in the present invention may also comprise, in combination with the anti-NR10 antibody mentioned above, other ingredients that enhance the treatment of inflammatory diseases.
  • the therapeutic agents of the present invention may also be used for preventive purposes.
  • the anti-NR10 antibody of the present invention may be prepared as formulations according to standard methods (see, for example, Remington's Pharmaceutical Science, latest edition, Mark Publishing Company, Easton, USA ). Further, they may contain pharmaceutically acceptable carriers and/or additives if necessary. For example, they may contain surfactants (for example, PEG and Tween), excipients, antioxidants (for example, ascorbic acid), coloring agents, flavoring agents, preservatives, stabilizers, buffering agents (for example, phosphoric acid, citric acid, and other organic acids), chelating agents (for example, EDTA), suspending agents, isotonizing agents, binders, disintegrators, lubricants, fluidity promoters, and corrigents.
  • surfactants for example, PEG and Tween
  • excipients for example, antioxidants (for example, ascorbic acid)
  • coloring agents for example, flavoring agents, preservatives, stabilizers
  • buffering agents for example, phosphoric acid, citric acid
  • the agents for preventing or treating inflammatory diseases of the present invention may contain other commonly used carriers.
  • Such carriers specifically include light anhydrous silicic acid, lactose, crystalline cellulose, mannitol, starch, carmelose calcium, carmelose sodium, hydroxypropylcellulose, hydroxypropylmethylcellulose, polyvinylacetaldiethylaminoacetate, polyvinylpyrrolidone, gelatin, medium chain fatty acid triglyceride, polyoxyethylene hydrogenated castor oil 60, sucrose, carboxymethylcellulose, corn starch, and inorganic salt.
  • the agents may also contain other low-molecular-weight polypeptides, proteins such as serum albumin, gelatin, and immunoglobulin, and amino acids such as glycine, glutamine, asparagine, arginine, and lysine.
  • the anti-NR10 antibody When the anti-NR10 antibody is prepared as an aqueous solution for injection, the anti-NR10 antibody may be dissolved in an isotonic solution containing, for example, physiological saline, dextrose, or other adjuvants.
  • the adjuvants may include, for example, D-sorbitol, D-mannose, D-mannitol, and sodium chloride.
  • solubilizing agents for example, alcohols (for example, ethanol), polyalcohols (for example, propylene glycols and PEGs), and non-ionic detergents (polysorbate 80 and HCO-50) may be used concomitantly.
  • alcohols for example, ethanol
  • polyalcohols for example, propylene glycols and PEGs
  • non-ionic detergents polysorbate 80 and HCO-50
  • anti-NR10 antibodies may be encapsulated in microcapsules (microcapsules made of hydroxymethylcellulose, gelatin, polymethylmethacrylate, and the like), and made into components of colloidal drug delivery systems (liposomes, albumin microspheres, microemulsions, nano-particles, and nano-capsules) (for example, see “ Remington's Pharmaceutical Science 16th edition” &, Oslo Ed. (1980 )).
  • colloidal drug delivery systems liposomes, albumin microspheres, microemulsions, nano-particles, and nano-capsules
  • methods for making sustained-release drugs are known, and these can be applied for anti-NR10 antibodies ( Langer et al., J. Biomed. Mater. Res. (1981) 15, 167-277 ; Langer, Chem. Tech. (1982) 12, 98-105 ; US Patent No. 3,773,919 ; European Patent Application (EP) No. 58,481 ; Sidman et al., Biopoly
  • compositions of the present invention can be administered either orally or parenterally, but are preferably administered parenterally.
  • the agents are administered to patients by injection or percutaneous administration.
  • Injections include, for example, intravenous injections, intramuscular injections, and subcutaneous injections, for systemic or local administration.
  • the agents may be given to sites where inflammation is to be suppressed, or areas surrounding the sites by local infusion, intramuscular injection in particular.
  • the administration methods can be properly selected according to the patient's age and condition.
  • the single-administration dose can be selected, for example, from within the range of 0.0001 to 100 mg of the active ingredient per kg body weight.
  • the dose of the active ingredient can be selected from within the range of 0.001 to 1,000 mg/kg body weight.
  • the single-administration dose preferably contains, for example, about 0.01 to 50 mg/kg body weight of the antibody of the present invention.
  • the dose of an agent for preventing or treating inflammatory diseases of the present invention is not limited to these examples.
  • Human NR10 (nucleotide sequence, SEQ ID NO: 75; amino acid sequence, SEQ ID NO: 76) was inserted into the expression vector pMacII, which expresses a protein under the control of mouse ⁇ -actin promoter (WO2005/054467), to prepare an expression vector for hNR10.
  • an expression vector for cynNR10 was constructed from cynomolgus monkey NR10 (nucleotide sequence, SEQ ID NO: 65; amino acid sequence, SEQ ID NO: 66).
  • the Helios Gene Gun Cartridge Kit (BIO-RAD) was used to produce a DNA cartridge for each DNA that allows immunization with 1 ⁇ g of DNA at one time.
  • mice Female; six weeks old at the beginning of immunization; Charles River Laboratories Japan
  • mice were immunized with human or cynomolgus monkey NR10 by the following procedure.
  • the mice were immunized with the DNA cartridge prepared with the hNR10 expression vector using the Helios Gene Gun System (BIO-RAD).
  • BIO-RAD Helios Gene Gun System
  • secondary immunization was performed by the Helios Gene Gun System (BIO-RAD) using the DNA cartridge prepared with the cynNR10 expression vector.
  • the third and subsequent immunizations were carried out at one-week intervals using the hNR10 and cynNR10 expression vectors alternately.
  • a human NR10 protein (extracellular domain) (Referential Example 4) diluted with PBS(-) was intravenously administered at 10 ⁇ g/head as the final immunization.
  • mouse spleen cells were fused with mouse myeloma P3X63Ag8U.1 cells (abbreviated as P3U1; ATCC CRL-1597) by a conventional method using PEG1500 (Roche Diagnostics).
  • the resulting fused cells i.e., hybridomas, were cultured in RPMI1640 supplemented with 10% FBS (hereinafter abbreviated as 10% FBS/RPMI1640).
  • the fused cells were suspended in a semisolid medium (StemCells), and cultured for selection as well as colonization of hybridomas.
  • HAT selection medium (10% FBS/ RPMI1640, 2 vol% of HAT 50x concentrate (Dainippon Pharmaceutical), and 5 vol% of BM-Condimed H1 (Roche Diagnostics)). After three to four days of culture, the culture supernatant was collected from each well to determine the concentration of mouse IgG in the supernatant.
  • the culture supernatants in which mouse IgG was detected were assessed for a neutralizing activity using a human IL-31-dependent cell line (hNR10/hOSMR/BaF3 cells; Referential Example 2), and several clones having a strong NR10-neutralizing activity were obtained ( Fig. 3 ).
  • Clones that suppress the human IL-31-induced growth of cells in a concentration-dependent manner and suppress the cynomolgus monkey IL-31-induced growth of cells cynNR10/cynOSMR/BaF3 cells; Referential Example 2) in a concentration-dependent manner were obtained ( Fig. 4 ).
  • RNAs were extracted from the hybridomas using RNeasy Mini Kits (QIAGEN), and cDNAs were synthesized from them using SMART RACE cDNA Amplification Kit (BD Biosciences).
  • Antibody variable region genes were isolated by PCR using PrimeSTAR HS DNA polymerase (TaKaRa), 10x Universal Primer A Mix attached to SMART RACE cDNA Amplification Kit (BD Biosciences), and primers designed for each antibody constant region (H chain, mIgG1-mot; L chain, mIgK-mot).
  • the nucleotide sequence of each isolated DNA fragment was determined with ABI PRISM 3730xL DNA Sequencer or ABI PRISM 3700 DNA Sequencer (Applied Biosystems), using BigDye Terminator Cycle Sequencing Kit (Applied Biosystems) according to the method described in the appended instruction manual.
  • the determined amino acid sequences of H chain and L chain variable regions in the mousse antibodies NS18, NS22, NS23, and NS33 were shown in Figs. 1 and 2 , respectively.
  • Each of the resulting H and L chain fragments was subjected to PCR using PrimeSTAR HS DNA Polymerase (TaKaRa) and the primer sets shown in Table 1.
  • the resulting amplified fragments were ligated with the constant region (human ⁇ 1 or ⁇ 2, and human ⁇ , respectively), and then inserted into an animal cell expression vector.
  • the nucleotide sequence of each DNA fragment was determined with ABI PRISM 3730xL DNA Sequencer or ABI PRISM 3700 DNA Sequencer (Applied Biosystems), using BigDye Terminator Cycle Sequencing Kit (Applied Biosystems) according to the method described in the appended instruction manual.
  • Human embryonic kidney cancer cell line HEK293H (Invitrogen) was suspended in DMEM (Invitrogen) supplemented with 10% fetal bovine serum (Invitrogen), and 10 ml of cells were seeded into dishes for adherent cells (10 cm in diameter; CORNING) at a cell density of 6 x 10 5 cells/ml. The cells were incubated in a CO 2 incubator (37°C, 5% CO 2 ) for one whole day and night. Then, the medium was removed by aspiration, and 6.9 ml of CHO-S-SFMII medium (Invitrogen) was added.
  • CHO-S-SFMII medium was added to the prepared plasmid DNA mixture (13.8 ⁇ g in total) to a volume of 700 ⁇ l. This was mixed with 20.7 ⁇ l of 1 ⁇ g/ml polyethyleneimine (Polysciences Inc.), and allowed to stand at room temperature for 10 minutes. The solution was added to the cells in each dish. The cells were incubated in a CO 2 incubator (37°C, 5% CO 2 ) for four to five hours. Then, 6.9 ml of CHO-S-SFMII medium (Invitrogen) was added, and the cells were incubated in a CO 2 incubator for three to four days. The culture supernatants were collected and then centrifuged (approx.
  • the activity of neutralizing hIL-31 was assessed using the hNR10/hOSMR/BaF3 cell line, which grows in an hIL-31 dose-dependent manner, as described below.
  • hNR10/hOSMR/BaF3 cells were prepared at 1.5 x 10 5 cells/ml using RPMI1640 medium (GIBCO) containing 10% FBS (MOREGATE) and 1% Penicillin-Streptomycin (Invitrogen).
  • hIL-31 R&D Systems
  • IL-31(+) was added to an aliquot of the cells to a final concentration of 4 ng/ml (IL-31(+); final conc.: 2 ng/ml).
  • the remaining cell suspension was usedasIL-31(-).
  • the purified NS22 was adjusted to 2 ⁇ g/ml using the medium, and eight serial dilutions were prepared at a common dilution ratio of 3 (final conc.: 1 ⁇ g/ml or less).
  • chimeric NS22 human ⁇ 1, ⁇
  • CORNING 96-well flat-bottom plates
  • the cells were cultured in a 5% CO 2 incubator at 37°C for two days.
  • 20 ⁇ l of a mixture of equal amounts of Cell Counting Kit-8 (Dojindo) and PBS was added to each well, and the absorbance (450 nm/620 nm) was measured (TECAN, SUNRISE CLASSIC). After the reaction was allowed to continue for two hours in a 5% CO 2 incubator at 37°C, the absorbance was measured again.
  • the neutralizing activity of NS22 was presented as an inhibition rate using a value obtained by subtracting the 0-hour value from the 2-hour value. The result showed that NS22 suppressed the IL-31-induced growth of the hNR10/hOSMR/BaF3 cell line in a concentration-dependent manner. This demonstrates that NS22 has a neutralizing activity against the human IL-31 signaling ( Fig. 5 ).
  • the IL-31-neutralizing activity was assessed as described below using the DU145 cell line (human prostate cancer cell line), in which IL-6 production is induced upon IL-31 stimulation.
  • DU145 cells were prepared at 2.5 x 10 5 cells/ml in MEM (Invitrogen) containing 10% FBS (MOREGATE), 2 mmol/l L-glutamine (Invitrogen), and 1 mmol/l sodium pyruvate (SIGMA), and 200- ⁇ l aliquots were dispensed into each well of 48-well plates (CORNING). The cells were incubated at 37°C under 5% CO 2 overnight. The purified chimeric NS22 (human ⁇ 1, ⁇ ) was diluted to 100 ⁇ g/ml with MEM containing 10% FBS, 2 mmol/l L-glutamine, and sodium pyruvate.
  • NS22 suppressed the IL-31-induced IL-6 production in the DU145 cell line in a concentration-dependent manner and thus demonstrated that NS22 had a neutralizing activity against the human IL-31 signaling ( Fig. 6 ).
  • Human IL-31 (R&D Systems) was labeled with FMAT Blue Monofunctional Reactive Dye (Applied Biosystems). 100 ⁇ l of hIL-31 prepared at 0.5 mg/ml using 50 mM sodium phosphate buffer (pH 8.0) was mixed with 5.25 ⁇ l of 25 nmoles FMAT Blue dissolved in DMSO (Junsei). After vortexing, the mixture was allowed to stand at room temperature for 15 minutes.
  • the FMAT Blue-conjugating reaction with hIL-31 was terminated by adding 5 ⁇ l of 1 M Tris-HCl (pH 7.4) and 1.1 ⁇ l of 10% Tween20, and then FMAT Blue-labeled hIL-31 and unreacted FMAT Blue were separated by gel filtration using Superdex 75 (GE Healthcare, 17-0771-01) column with 0.1% Tween20/PBS developing solution.
  • Antibodies were assessed for the activity of inhibiting the IL-31/NR10 binding by using hNR10-expressing CHO cells as described below.
  • NS22 and NA633 (the constant region of each is ⁇ 1, ⁇ ) were diluted at an appropriate concentration using Assay buffer (10 mM HEPES, 140 mM NaCl, 2.5 mM CaCl 2 , 3 mM MgCl 2 , 2% FBS, 0.01 % NaN 3 ), and then seven serial dilutions were prepared at a common dilution ratio of 2. The dilutions were added at 40 ⁇ l/well to plates (96-Well FMAT Plates; Applied Biosystems). Then, FMAT Blue-labeled hIL-31 was diluted 400 times with Assay buffer and added at 20 ⁇ l/well.
  • Assay buffer 10 mM HEPES, 140 mM NaCl, 2.5 mM CaCl 2 , 3 mM MgCl 2 , 2% FBS, 0.01 % NaN 3
  • Assay buffer 10 mM HEPES, 140 mM NaCl, 2.5 mM CaCl 2
  • the antibody NS22 purified from a hybridoma culture supernatant was labeled with FMAT Blue (Applied Biosystems, 4328853). 170 ⁇ l of NS22 prepared at 1 mg/ml in PBS was mixed with 17 ⁇ l of 1 M NaHCO 3 solution and 3.4 ⁇ l of FMAT Blue (17 nmoles) dissolved in DMSO. After vortexing, the mixture was allowed to stand at room temperature for 30 minutes.
  • the FMAT Blue conjugating reaction with NS22 was terminated by adding 8 ⁇ l of 1 M Tris-HCl (pH 7.4) and 1.9 ⁇ l of 1% Tween 20, and then FMAT Blue-labeled NS22 (FMAT Blue-NS22) and unreacted FMAT Blue were separated by gel filtration using Superdex 75 (GE Healthcare, 17-0771-01) column with 0.01% Tween20/PBS developing solution.
  • Each antibody was examined for inhibition of the binding of the prepared FMAT Blue-NS22 to hNR10-expressing CHO cells (Referential Example 3) using the 8200 Cellular Detection System (Applied Biosystems, 4342920).
  • the chimeric anti-NR10 antibodies (the constant region of each is ⁇ 1, ⁇ ) were added at various concentrations to each well containing 7500 cells and 8.8 x 10 -2 ⁇ g/ml FMAT Blue-NS22. The cells were allowed to stand in the dark for four hours, and then the fluorescent signal from FMAT Blue bound to the cells was measured.
  • the reaction was carried out in 10 mM Hepes-KOH containing 2.5 mM CaCl 2 , 3 mM MgCl 2 , 140 mM NaCl, 2% FBS, and 0.01% NaNO 3 .
  • the result is shown in Fig. 8 .
  • the fluorescence value FL1 which represents the binding of FMAT Blue-NS22 to NR10-expressing cells, was reduced with the increase in the concentration of antibody NS22 or NS23.
  • FL1 was hardly reduced with the increase in the concentration of antibody NA633 (Referential Example 6) ( Fig. 8 ).
  • variable regions of mouse NS22 antibody were compared with human germline sequences.
  • FR sequences used for humanization are summarized in Table 2. CDRs and FRs were determined based on the Kabat numbering.
  • the humanized variable region sequences of H chain composed of FR1, FR2, FR3_1, and FR4, and composed of FR1, FR2, FR3_2, and FR4, which are listed in Table 2, are designated as H0-VH (SEQ ID NO: 50) and H1-VH (SEQ ID NO: 112), respectively.
  • sequence of L chain composed of FR1, FR2, FR3, and FR4 is designated as L0 (SEQ ID NO: 52).
  • Synthetic oligo DNAs were designed for each of the H and L chains to construct the variable regions of humanized NS22 in which the CDRs of NS22 are grafted onto the FRs used for humanization.
  • the respective synthetic oligo DNAs were mixed, and then subjected to assembly PCR to construct a gene encoding the variable region of humanized NS22.
  • the assembly PCR was carried out using KOD-Plus (TOYOBO) according to the following conditions. A reaction mixture containing 10 pmol synthetic oligo DNAs and the appended PCR Buffer, dNTPs, MgSO 4 , and KOD-Plus was heated at 94°C for five minutes.
  • the mixture was then subjected to two PCR cycles of 94°C for two minutes, 55°C for two minutes, and 68°C for two minutes. Then, 10 pmol each of a primer in which a restriction site and Kozak sequence has been added to the 5' end of the variable region, and a primer in which a restriction site has been added to the 3' end of the variable region, was added and subjected to 35 PCR cycles of 94°C for 30 seconds, 55°C for 30 seconds, and 68°C for one minute to yield a amplified fragment. The resulting amplified fragment was cloned into TOPO TA Cloning vector (TOYOBO), and its nucleotide sequence was determined by sequencing.
  • TOPO TA Cloning vector TOPO TA Cloning vector
  • the constructed variable regions were combined with the constant regions to prepare HO-SKSC (SEQ ID NO: 54) and L0 (SEQ ID NO: 56).
  • the resulting construct was inserted into an expression vector capable of expressing the inserted gene in animal cells.
  • the nucleotide sequence of each DNA fragment was determined using BigDye Terminator Cycle Sequencing Kit (Applied Biosystems) with ABI PRISM 3730xL DNA Sequencer or ABI PRISM 3700 DNA Sequencer (Applied Biosystems) according to the method described in the appended instruction manual.
  • H1-SKSC (SEQ ID NO: 130) was generated by substituting the glutamine (E) at Kabat-numbering position 73 in FR3 of H0-SKSC (SEQ ID NO: 54) with lysine (K).
  • the mutant was prepared using commercially available QuikChange Site-Directed Mutagenesis Kit (Stratagene) according to the appended instruction manual.
  • Antibody expression was performed by the method described below.
  • Human fetal renal cancer cell-derived cell line HEK293H (Invitrogen) was suspended in DMEM (Invitrogen) containing 10% fetal bovine serum (Invitrogen), and 10 ml of cells at a density of 5-6 x 10 5 cells/ml was seeded onto dishes for adherent cells (10 cm in diameter; CORNING).
  • the cells were incubated in a CO 2 incubator (37°C, 5% CO 2 ) for one whole day and night. Then, the medium was removed by aspiration, and 6.9 ml of CHO-S-SFMII medium (Invitrogen) was added to the cells.
  • the prepared plasmid DNA mixture (13.8 ⁇ g in total) was mixed with 20.7 ⁇ l of 1 ⁇ g/ml polyethyleneimine (Polysciences Inc.) and 690 ⁇ l of CHO-S-SFMII medium, and allowed to stand at room temperature for 10 minutes. The mixture was added to the cells in each dish, and the cells were incubated in a CO 2 incubator (5% CO 2 , 37°C) for four to five hours. Then, 6.9 ml of CHO-S-SFMII medium (Invitrogen) was added, and the cells were incubated in a CO 2 incubator for three days. The culture supernatant was collected and centrifuged (approx. 2000 g, five minutes, room temperature) to remove the cells. The supernatant was then sterilized by filtration through 0.22- ⁇ m filter MILLEX ® -GV (Millipore). Each sample was stored at 4°C until use.
  • rProtein A Sepharose TM Fast Flow 50 ⁇ l of rProtein A Sepharose TM Fast Flow (Amersham Biosciences) suspended in TBS was added to the obtained culture supernatant, and mixed by inversion at 4°C for four hours or more. The solution was transferred to 0.22- ⁇ m filter cup of Ultrafree ® -MC (Millipore). After three washes with 500 ⁇ l of TBS, rProtein A Sepharose TM resin was suspended in 100 ⁇ l of aqueous solution of 50 mM sodium acetate (pH 3.3), and allowed to stand for three minutes to elute the antibody. The solution was immediately neutralized by adding 6.7 ⁇ l of 1.5 M Tris-HCl (pH 7.8).
  • the elution was performed twice and 200 ⁇ l of purified antibody was obtained. 2 ⁇ l of the antibody-containing solution was subjected to ND-1000 Spectrophotometer (NanoDrop)(Thermo Scientific NanoDrop TM 1000 Spectrophotometer (Thermo Scientific)) or 50 ⁇ l was subjected to Spectrophotometer DU-600 (BECKMAN) to measure absorbance at 280 nm, and the antibody concentration was calculated by the method of Pace et al. (Protein Science (1995) 4: 2411-2423 ).
  • Antibodies were assessed for the activity of inhibiting the IL-31/NR10 binding by using hNR10-expressing CHO cells as described below.
  • the chimeric NS22 antibody and NS22_H0L0 (H chain, H0-SKSC/SEQ ID NO: 54; L chain, L0/SEQ ID NO: 56) were diluted at an appropriate concentration using Assay buffer (10 mM HEPES, 140 mM NaCl, 2.5 mM CaCl 2 , 3 mM MgCl 2 , 2% FBS, 0.01% NaN 3 , pH7.4), and further eight serial dilutions were prepared at a common dilution ration of 2.
  • humanized NS22 antibodies H0L0 H chain, H0-SKSC/SEQ ID NO: 54; L chain, L0/SEQ ID NO: 56
  • H1L0 H chain, H1-SKSC/SEQ ID NO: 130; L chain, L0/SEQ ID NO: 56
  • FRs used for H0L0 and H1L0 can be used for humanization.
  • the heterogeneity was assessed by cation exchange chromatography.
  • the prepared antibodies were assessed for heterogeneity using ProPac WCX-10 (Dionex) column, 20 mM sodium acetate (pH 5.0) as mobile phase A, and 20 mM sodium acetate/1M NaCl (pH 5.0) as mobile phase B, with an appropriate flow rate and gradient.
  • the result of assessment by cation exchange chromatography (IEC) is shown in Fig. 10 .
  • the heterogeneity was increased by conversion of the constant region from IgG1 to IgG2 in the anti-IL-31 receptor antibody, and the heterogeneity can be reduced by conversion of the constant region to M14 or M58 in any antibody.
  • H0L0-IgG1 H chain: H0-IgG1/SEQ ID NO: 133; L chain: L0/SEQ ID NO: 56
  • H0L0-M58 H chain: H0-M58/SEQ ID NO: 136; L chain L0/SEQ ID NO: 56
  • Each mutant was produced by the method described in Example 4 or by assembly PCR.
  • oligo DNAs are synthesized based on forward and reverse sequences including an altered site. Forward oligo DNA including an altered site and reverse oligo DNA binding to the vector in which the gene to be altered was inserted were combined, and reverse oligo DNA including an altered site and forward oligo DNA binding to the vector in which the gene to be altered was inserted were combined.
  • PCR was carried out using PrimeSTAR (Takara) to produce 5'-end and 3'-end fragments including the altered site. The two fragments were assembled by assembly PCR to produce each mutant. The produced mutant was inserted into an expression vector capable of expressing the insert gene in animal cells. The nucleotide sequence of the resulting expression vector was determined by a method known to those skilled in the art. Antibodies were produced and purified by the method described in Example 4.
  • H0L0 H chain, H0-SKSC/SEQ ID NO: 54; L chain, L0/SEQ ID NO: 56
  • altered sites capable of reducing the isoelectric point of the variable region were examined. Screening of mutation sites in the variable regions predicted from the three-dimensional structure model revealed mutation sites that would decrease the isoelectric point of the variable regions without significantly reducing its binding to NR10.
  • Each variant was tested for the activity of inhibiting the hIL-31/hNR10 binding by using FMAT.
  • the test was carried out according to the method as described in Example 4. As shown in Fig. 11 , the competition activity of each variant was not greatly reduced as compared to that of H0L0.
  • Asterisk (*) in Table 4 above indicates a site that was not relevant to the isoelectric point but altered for conversion into a human sequence.
  • Hp3Lp15 H chain: Hp3-SKSC/SEQ ID NO: 151; L chain: Lp15/SEQ ID NO: 152).
  • Affinity for NR10, isoelectric point, and plasma retention in mice were compared between Hp3Lp15 and H0L0.
  • Isoelectric focusing was performed by the following method.
  • Phast-Gel Dry IEF gel was swollen in Phastsystem Cassette (Amersham Biosciences) for about 30 minutes using the swelling solution shown below. MilliQ water 1.5 ml Pharmalyte 5-8 for IEF (Amersham Biosciences) 100 ⁇ l
  • Electrophoresis was carried out in PhastSystem (Amersham Biosciences) using the swollen gel according to the program indicated below. The samples were loaded onto the gel in Step 2. Calibration Kit for pI (Amersham Biosciences) was used as a pI marker. Step 1: 2000 V 2.5 mA 3.5 W 15°C 75 Vh Step 2: 200 V 2.5 mA 3.5 W 15°C 15 Vh Step 3: 2000 V 2.5 mA 3.5 W 15°C 410 Vh
  • the gel was fixed with 20% TCA, and then silver-stained using the Silver Staining Kit, Protein (Amersham Biosciences), according to the protocol attached to the kit. After staining, the isoelectric point of the sample (the whole antibody) was calculated from the known isoelectric points of the pI markers.
  • H0L0 and Hp3Lp15 were compared in normal mice.
  • a single dose of H0L0 or Hp3Lp15 was intravenously administered at 1 mg/kg to mice (C57BL/6J, Charles River Japan, Inc.) to compare the time course of the plasma concentration.
  • the plasma concentrations were determined by ELISA. Appropriate concentrations of a calibration sample and test plasma samples were dispensed into immunoplates (Nunc-Immuno Plate, MaxiSorp (Nalge Nunc International)) coated with anti-human IgG (Fc-specific) antibody (Sigma). The samples were allowed to stand at room temperature for one hour.
  • AUC and systemic clearance (CL) were calculated from the obtained time-course data of the plasma concentration using the pharmacokinetics analysis software WinNonlin (Pharsight). The parameters are shown in Table 6. AUC and the clearance of Hp3Lp15 after the intravenous administration were increased by about 14% and reduced by about 12%, respectively, as compared to H0L0. Thus, it was demonstrated that Hp3Lp15, in which the isoelectric point of H0L0 has been reduced, had improved pharmacokinetics.
  • Table 6 AUC( ⁇ g ⁇ d/kg) CL(ml/d/kg) Mean SD Mean SD H0L0 281.8 13.1 3.6 0.2 Hp3Lp15 321.1 26.1 3.1 0.3
  • SKSC SEQ ID NO: 62
  • M58 SEQ ID NO: 128, constant regions prepared in Referential Examples 7 and 9, were combined with Hp3 (Hp3-VH/SEQ ID NO: 167), a variable region prepared in Example 7, to produce Hp3-M58 (SEQ ID NO: 240) and Hp3-SKSC (SEQ ID NO: 151) as H chains.
  • the prepared H chains were combined with Lpl5 (Lp15/SEQ ID NO: 152), an L chain prepared in Example 7, to produce Hp3Lp15-SKSC (H chain, Hp3-SKSC/SEQ ID NO: 151; L chain, Lp15/SEQ ID NO: 152) and Hp3Lp15-M58 (H chain, Hp3-M58/SEQ ID NO: 240; L chain, Lp15/SEQ ID NO: 152).
  • Hp3Lp15-SKSC H chain, Hp3-SKSC/SEQ ID NO: 151; L chain, Lp15/SEQ ID NO: 152
  • Hp3Lp15-M58 H chain, Hp3-M58/SEQ ID NO: 240; L chain, Lp15/SEQ ID NO: 152
  • Each antibody was expressed and purified by the method described in Example 4.
  • H0L0-SKSC H chain, H0-SKSC/SEQ ID NO: 54; L chain, L0/SEQ ID NO: 56
  • H0L0-M58 H chain, H0-M58/SEQ ID NO: 136; L chain, L0/SEQ ID NO: 56
  • H0L0-IgG2 H chain, H0-IgG2/SEQ ID NO: 134; L chain, L0/SEQ ID NO: 56
  • Fig. 18 The antibodies produced as described above, H0L0-SKSC (H chain, H0-SKSC/SEQ ID NO: 54; L chain, L0/SEQ ID NO: 56) prepared using the constant region SKSC (SEQ ID NO: 62) described in Referential Example 7, and H0L0-M58 (H chain, H0-M58/SEQ ID NO: 136; L chain, L0/SEQ ID NO: 56) and H0L0-IgG2 (H chain, H0-IgG2/SEQ ID NO: 134; L chain, L0/SEQ ID NO:
  • Antibodies used for pharmaceuticals have heterogeneity even though they are monoclonal antibodies obtained from clones derived from single antibody-producing cells. Such antibody heterogeneity is known to result from modification such as oxidation or deamidation, and to be increased during long-term storage or upon exposure to stress conditions, such as heat stress or light stress (see “ Heterogeneity of Monoclonal Antibodies", Journal of pharmaceutical sciences, vol. 97, No. 7, 2426-2447 ). However, when an antibody is developed as a pharmaceutical, physical properties of the protein, particularly homogeneity and stability, are highly important. Thus, it is desired that the heterogeneity of desired/related substances be reduced and the substance be composed of a single substance as much as possible. In this context, the experiment described below was conducted to assess the antibody heterogeneity under stress conditions and to reduce the heterogeneity.
  • H0L0 H chain, H0-SKSC/SEQ ID NO: 54; L chain, L0/SEQ ID NO: 56
  • the prepared accelerated sample and non-accelerated sample (initial) were analyzed by cation exchange chromatography using the method described below.
  • Ha355L0 H chain, Ha355-SKSC/SEQ ID NO: 242; L chain, L0/SEQ ID NO: 56
  • Ha356L0 H chain, Ha356-SKSC/SEQ ID NO: 243; L chain, L0/SEQ ID NO: 56
  • Ha360L0 H chain, Ha360-SKSC/SEQ ID NO: 244; L chain, L0/SEQ ID NO: 56
  • Ha362L0 H chain, Ha362-SKSC/SEQ ID NO: 245; L chain, L0/SEQ ID NO: 56).
  • Each of the identified antibodies was expressed and purified by the method described in Example 4. As with H0L0, a accelerated sample of each prepared antibody was prepared, and analyzed by cation exchange chromatography. The result is shown in Fig. 19 .
  • the result showed that the generation of the basic peak increased after acceleration was reduced in the modified antibody containing a substitution of aspartic acid with glutamic acid at position 101 in the H chain, as compared to H0L0.
  • the modified antibodies were assessed for the biological activity by the method described in Example 2 using BaF/NR10. The result is shown in Fig. 20 . As shown in Fig. 20 , the biological activities of the modified antibodies were comparable to or stronger than that of H0L0.
  • a library in which mutations were introduced into CDR sequences was constructed and examined to improve the affinity of H0L0 for NR10.
  • mutations that improve the affinity for NR10 were found. The mutations are shown in Table 8.
  • Examples of combinations of these affinity-improving mutations with the isoelectric point-lowering mutations generated in Example 7 include, for example, Ha401La402 (H chain, Ha401-SKSC/SEQ ID NO: 255; L chain, La402/SEQ ID NO: 256) and H17L11 (H chain, H17-M58/SEQ ID NO: 222; L chain, L11/SEQ ID NO: 236). Each variant was produced and purified by the method described in Example 4.
  • Ha401La402 H chain, Ha401-SKSC/SEQ ID NO: 255; L chain, La402/SEQ ID NO: 256
  • H0L0 H chain, H0-SKSC/SEQ ID NO: 54; L chain, L0/SEQ ID NO: 56
  • the result of affinity measurement is shown in Table 10, and the biological activity determined using BaF/NR10 is shown in Fig. 21 .
  • H17L11 H chain, H17-M58/SEQ ID NO: 222; L chain, L11/SEQ ID NO: 236) was assessed for its affinity for NR10 and its biological activity by the method described in Example 7 and the method using BaF/NR10 as described in Example 2, respectively, and they were compared to those of H0L0 (H chain, H0-M58/SEQ ID NO: 136; L chain, L0/SEQ ID NO: 56).
  • the result of affinity measurement is shown in Table 11, and the biological activity determined using BaF/NR10 is shown in Fig. 22 .
  • T-cell epitopes present in the variable region sequence of H0L0 were analyzed using TEPITOPE ( Methods 2004 Dec; 34(4): 468-75 ).
  • CDR1 of the H chain was predicted to have many T-cell epitopes that bind to HLA (i.e. have sequences with a high immunogenicity risk).
  • TEPITOPE analysis was carried out to examine substitutions that would reduce the immunogenicity risk of the H chain CDR1.
  • the immunogenicity risk was found to be greatly reduced by substituting isoleucine at position 33 in kabat numbering with alanine (A) (Table 12).
  • the antibody was assessed for the affinity for NR10 and the biological activity by the method described in Referential Example 10 and the method using BaF/NR10 as described in Example 2, respectively, and they were compared to those of H0L0 (H chain, H0-M58/SEQ ID NO: 136; L chain, L0/SEQ ID NO: 56).
  • H0L0 H chain, H0-M58/SEQ ID NO: 136; L chain, L0/SEQ ID NO: 56.
  • the result of affinity measurement is shown in Table 13, and the biological activity determined using BaF/NR10 is shown in Fig. 23 . Both affinity and biological activity were shown to be almost equal to those of H0L0.
  • Threonine (T) present at kabat-numbering position 25 in CDR1 of the L chain corresponds to alanine (A) or serine (S) in the germline sequence.
  • Threonine (T) at position 25 corresponds to alanine (A) or serine (S) in the germline sequence.
  • T threonine
  • S serine
  • Table 14 the above substitution was added to L12 to produce L17 (SEQ ID NO: 238).
  • the produced L17 was combined with H0 to produce H0L17 (H chain, H0-M58/SEQ ID NO: 136; L chain, L17/SEQ ID NO: 238).
  • Each variant was produced and purified by the method described in Example 4.
  • Each variant was assessed for the affinity for NR10 and the biological activity by the method described in Referential Example 10 and the method using BaF/NR10 as described in Example 2, respectively, and they were compared to those of H0L0 (H chain, H0-M58/SEQ ID NO: 136; L chain, L0/SEQ ID NO: 56) and H0L12 (H chain, H0-M58/SEQ ID NO: 136; L chain, L12/SEQ ID NO: 237). Since L12 contains a sequence that improves the affinity, it exhibits about two times higher affinity than H0L0. The result of affinity measurement is shown in Table 15, and the biological activity determined using BaF/NR10 is shown in Fig. 24 .
  • Variable regions of NS22 variants were prepared by combining the multiple mutations that reduce the pI, increase the affinity, suppress the degradation of H chain, and reduce the immunogenicity risk, all of which were found in the above Examples, in H0 (H0-M58/SEQ ID NO: 136), H1 (H1-M58/SEQ ID NO: 257), or L0 (L0/SEQ ID NO: 56), and subjected to various screening procedures.
  • H28L17 H chain, H28-M58/SEQ ID NO: 224; L chain, L17/SEQ ID NO: 238), H30L1.7 (H chain, H30-M58/SEQ ID NO: 225; L chain, L17/SEQ ID NO: 238), H34L17 (H chain, H34-M58/SEQ ID NO: 226, L chain, L17/SEQ ID NO: 238), H42L17 (H chain, H42-M58/SEQ ID NO: 227; L chain, L17/SEQ ID NO: 238), H44L17 (H chain, H44-M58/SEQ ID NO: 228; L chain, L17/SEQ ID NO: 238), H46L17 (H chain, H46-M58/SEQ ID NO: 229; L chain, L17/SEQ ID NO: 238), H57L17 (H chain, H57-M58/SEQ ID NO: 230; L chain, L17/SEQ ID NO: 238)
  • Each variant was assessed for the affinity for NR10 and the biological activity by the method described in Referential Example 10 and the method using BaF/NR10 as described in Example 2, respectively, and they were compared to those of H0L0 (H chain, H0-M58/SEQ ID NO: 136; L chain, L0/SEQ ID NO: 56).
  • the result of affinity measurement is shown in Table 16, and the biological activity determined using BaF/NR10 is shown in Fig. 25-1 and 25-2 . Both affinity and biological activity of each antibody were shown to be almost equal to or greater than those of H0L0.
  • the human/mouse wild-type and chimeric antigens (hhh, mmm, hhm, mmh, hmm, mhm, and mhh) were purified from culture supernatants by Ni-NTA Superflow column chromatography. Specifically, 1 ml of Ni-NTA Superflow (QIAGEN) was loaded onto Poly-Prep Empty Column (BioRad), and 30 ml of each culture supernatant was added thereto.
  • D-PBS Dulbecco's phosphate-buffered saline
  • the column was eluted with D-PBS containing 150 mM sodium chloride and 250 mM imidazole.
  • the eluted fractions were buffer exchanged with D PBS and concentrated using Amicon-Ultra (Millipore) with a molecular weight cut-off of 10K.
  • Each of the prepared human/mouse wild-type and chimeric antigens was electrophoresed at 0.5 ⁇ g/lane on three 4-20% polyacrylamide gels (Daiichi Pure Chemicals Co.).
  • the proteins were electro-transferred onto PVDF membranes (Millipore) in a semi-dry blotting apparatus, and the membranes were blocked with TBS containing 5% skim milk.
  • H44M58L17 detection system for humanized anti-human NR10 antibody
  • ND41 detection system for mouse anti-human NR10 antibody
  • anti-Myc antibody SuraCruz, Cat.#sc-789
  • Alkaline phosphatase-labeled goat anti-human IgG ⁇ (BIOSOURCE, Cat. #AHI0305) was used to detect humanized anti-human NR10 antibody; alkaline phosphatase-labeled goat anti-mouse IgG (SantaCruz, Cat. #sc-2008) was used to detect mouse anti-human NR10 antibody; and alkaline phosphatase-labeled goat anti-rabbit IgG (SantaCruz, Cat. #sc-2057) was used to detect Myc tag. The reaction was carried out at room temperature for one hour.
  • TBS Tris-buffered saline
  • TBS Tris buffered saline
  • the binding was detected only for hhh, hhm, and hmm, which are NR10 extracellular domains.
  • cynomolgus monkey NR10 and OSMR genes were isolated. Primers were designed based on published information of Rhesus monkey genome and others, and the NR10 and OSMR genes were successfully amplified by PCR from cynomolgus monkey pancreatic cDNA.
  • sequences of the isolated cynomolgus monkey NR10, OSMR, and IL-31 genes are shown in SEQ ID NOs: 65, 69, and 67, respectively, and the amino acid sequences of cynomolgus monkey NR10, OSMR, and IL-31 are shown in SEQ ID NOs: 66, 70, and 68, respectively.
  • the full-lenglth human NR10 cDNA (SEQ ID NO: 75) was inserted into the expression vector pCOS1 ( Biochem. Biophys. Res. Commun. 228, p838-45, 1996 ), and the resulting vector was named pCosNR10.3.
  • An oncostatin M receptor cDNA (OSMR, GenBank accession No. NM003999) was isolated by PCR from a human placental library, and the expression vector pCos1-hOSMR was constructed in the same manner. 10 ⁇ g each of the vectors were simultaneously introduced into mouse IL-3-dependent pro-B cell-derived cell line Ba/F3 by electroporation (BioRad Gene Pulser, 960 ⁇ F, 0.33 kV).
  • IL-31 human IL-31 (R&D Systems) was added, and the cells were cultured to obtain a cell line (hNR10/hOSMR/BaF3 cell) that proliferates in an IL-31-dependent manner. Furthermore, the cynomolgus monkey IL-31 gene (SEQ ID NO: 67) was inserted into a mammalian cell expression vector and introduced into CHO cell line DG44. The resulting culture supernatant was obtained as cynomolgus monkey IL-31.
  • cynomolgus monkey NR10 and OSMR genes were inserted into the expression vector pCOS1 and expressed in Ba/F3 cells, and a cynomolgus monkey IL-31-dependent cell line (cynNR10/cynOSMR/BaF3 cell) was established using the culture supernatant described above.
  • cytoplasmic domain-lacking human NR10 SEQ ID NO: 73
  • cytoplasmic domain-lacking cynomolgus monkey NR10 SEQ ID NO: 71
  • the genes for cytoplasmic domain-lacking human NR10 SEQ ID NO: 73
  • cytoplasmic domain-lacking cynomolgus monkey NR10 SEQ ID NO: 71
  • the resulting vectors were linearized with a restriction enzyme, and then introduced into CHO cell line DG44 by electroporation (BioRad Gene Pulser, 25 ⁇ F, 1.5 kV).
  • NR10-expressing cells were selected and established by FCM analysis using anti-human NR10 antibody.
  • amino acid sequence encoded by the nucleotide sequence of cytoplasmic domain-lacking human NR10 gene is shown in SEQ ID NO: 74
  • amino acid sequence encoded by the nucleotide sequence of cytoplasmic domain-lacking cynomolgus monkey NR10 gene is shown in SEQ ID NO: 72.
  • the human NR10 cDNA was used as a template to amplify only the extracellular domain by PCR.
  • the amplified region was then fused to a FLAG tag sequence at the C terminus and inserted to a mammalian cell expression vector.
  • Ten ⁇ g of the linearized vector was introduced into Chinese hamster ovary cell line DG44 by electroporation (BioRad Gene PulserII, 25 ⁇ F, 1.5 kV). A cell line showing high level expression was obtained.
  • the supernatant of the cell line cultured on a large scale was purified using anti-FLAG antibody column (Sigma) and gel filtration to obtain soluble NR10.
  • the nucleotide sequence of soluble NR10 is shown in SEQ ID NO: 77, and the amino acid sequence is shown in SEQ ID NO: 78.
  • mice were immunized with human NR10 protein (extracellular domain) (described in Referential Example 4), and hybridomas were prepared by a conventional method. The culture supernatants of these hybridomas were assessed for the neutralizing activity using the human IL-31-dependent cell line (hNR10/hOSMR/BaF3 cell) described in Referential Example 2, and thereby NA633 which has an NR10-neuralizing activity was obtained.
  • DNA immunization was carried out by He gas-driven gene gun using a mammalian expression vector carrying the full-length human NR10 gene (SEQ ID NO: 75), and hybridomas were prepared by a conventional method.
  • the culture supernatants of these hybridomas were assessed for the neutralizing activity using the human IL-31 -dependent cell line (hNR10/hOSMR/BaF3 cell) described in Referential Example 2, and thereby ND41 which has an NR10-neuralizing activity was obtained.
  • the amino acid sequences of heavy chain and light chain variable regions of NA633 are shown in SEQ ID NOs: 104 and 108, respectively.
  • the amino acid sequences of CDR1, CDR2, and CDR3 of the heavy chain variable region of NA633 are shown in SEQ ID NOs: 105, 106, and 107, respectively, while those of CDR1, CDR2, and CDR3 of the light chain variable region are shown in SEQ ID NOs: 109, 110, and 111, respectively.
  • a chimeric antibody between these mouse variable regions and human constant region was produced by a conventional method.
  • the NS22 antibody is an NR10-neutralizing antibody
  • its binding to Fc ⁇ receptor may be unfavorable in consideration of the immunogenicity and adverse effects.
  • a possible method for reducing the binding to Fe ⁇ receptor is to select IgG2 or IgG4 instead of IgG1 as the isotype of the constant region ( Ann Hematol. 1998 Jun; 76(6): 231-48 .). From the viewpoint of Fc ⁇ receptor I and retention in plasma, IgG2 has been considered more desirable than IgG4 ( Nat Biotechnol. 2007 Dec; 25(12): 1369-72 ). Meanwhile, when an antibody is developed as a pharmaceutical, properties of the protein, particularly homogeneity and stability, are highly important.
  • the IgG2 isotype has been reported to have very high heterogeneity resulting from the disulfide bonds in the hinge region ( J Biol Chem. 2008 Jun 6; 283(23): 16206-15 .). It is not easy and would be more costly to manufacture it as pharmaceutical in a large scale while maintaining difference in the heterogeneity of desired/related substances among products resulting from the above. Accordingly, it is desired that the substance be composed of a single substance as much as possible. Thus, when antibodies of IgG2 isotype are developed as pharmaceuticals, it is preferred to reduce the heterogeneity resulting from disulfide bonds, without lowering the stability.
  • SKSC SEQ ID NO: 62
  • EU numbering Sequences of proteins of immunological interest, NIH Publication No.91-3242
  • altering cysteine at EU-numbering position 219 in the H-chain upper hinge to serine could reduce the heterogeneity without decreasing the stability.
  • huPM1-SC SEQ ID NO: 157
  • huPM1-CS SEQ ID NO: 158
  • huPM1-IgG1 SEQ ID NO: 159
  • huPM1-IgG2 SEQ ID NO: 160
  • huPM1-SKSC SEQ ID NO: 161
  • H chain variable region huPM1-VH/SEQ ID NO: 155
  • L chain variable region huPM1-VL/SEQ ID NO: 156 Cancer Res. 1993 Feb 15;53(4): 851-6 .
  • the antibodies were compared to each other in terms of the heterogeneity.
  • the heterogeneity of huPM1-IgG1, huPM1-IgG2, huPM1-SC huPM1-CS, and huPM1-SKSC was assessed by cation exchange chromatography.
  • the chromatography was carried out using a ProPac WCX-10 (Dionex) column, 20 mM sodium acetate (pH 5.0) as mobile phase A, and 20 mM sodium acetate/1M NaCl (pH 5.0) as mobile phase B, with an appropriate flow rate and gradient.
  • the result of assessment by cation exchange chromatography is shown in Fig. 12 .
  • Tm value thermal denaturation midpoint temperature
  • DSC differential scanning calorimetry
  • VP-DSC Microcal
  • Tm value serves as an indicator of stability.
  • a higher thermal denaturation midpoint temperature (Tm value) is preferred ( J Pharm Sci. 2008 Apr; 97(4): 1414-26 .).
  • huPM1-IgG1, huPM1-IgG2, huPM1-SC, huPM1-CS, and huPM1-SKSC were dialyzed against a solution of 20 mM sodium acetate/150 mM NaCl (pH 6.0) (EasySEP; TOMY), and DSC measurement was carried out using about 0.1 mg/ml of protein at a heating rate of 1°C/min between 40 and 100°C.
  • the denaturation curves obtained by DSC are shown in Fig. 13 .
  • the Tm values of the Fab domains are listed in Table 17 below. Table 17 Name Tm/°C huPM1-IgG1 94.8 huPM1-IgG2 93.9 huPM1-SC 86.7 huPM1-CS 86.4 huPM1-SKSC 93.7
  • the Tm values of huPM1-IgG1 and huPM1-IgG2 were almost the same, namely, about 94°C (IgG2 was lower by about 1°C). Meanwhile, the Tm values of huPM1-SC and huPM1-CS were about 86°C, which was significantly lower than those of huPM1-IgG1 and huPM1-IgG2. On the other hand, the Tm value of huPM1-SKSC was about 94°C, and almost the same as huPM1-IgG1 and huPM1-IgG2.
  • huPM1-SKSC in which cysteine in the CH1 domain have also been altered to serine may be more preferred in the development of pharmaceuticals.
  • the significant decrease in Tm value of huPM1-SC and huPM1-CS as compared to IgG2 may be due to the disulfide-bonding pattern of huPM1-SC and huPM1-CS that is different from that of IgG2.
  • the denaturation peak for the Fab domain was sharp in huPM1-IgG1 and huPM1-SKSC, while it was broader in huPM1-SC and huPM1-CS than the above two, and huPM1-IgG2 gave a shoulder peak on the lower temperature side of the Fab domain denaturation peak.
  • the denaturation peak in DSC generally becomes sharp in the case of a single component, but may become broad when two or more components with different Tm values (namely, heterogeneity) are present.
  • huPM1-IgG2 huPM1-SC, and huPM1-CS contained two or more components, and the heterogeneity of natural IgG2 was not reduced in huPM1-SC and huPM1-CS.
  • cysteines present in both the hinge region and the CH1 domain are involved in the heterogeneity of natural IgG2, and it is necessary to alter not only cysteine in the hinge region but also that in the CH1 domain to decrease the heterogeneity on DSC.
  • SC and CS which are constant regions in which only cysteine in the hinge region has been substituted with serine, may be insufficient from the viewpoint of heterogeneity and stability, and that it is only possible to significantly reduce the heterogeneity while maintaining the stability comparable to IgG2 by additionally substituting cysteine at EU-numbering position 131 in the CH1 domain with serine.
  • Such constant regions include SKSC.
  • the residues at EU-numbering positions 233, 234, 235, and 236 are of non-binding type, while the residues at EU-numbering positions 327, 330, and 331 are different from those of IgG4, which are of non-binding type.
  • it is necessary to alter the amino acids at EU-numbering positions 327, 330, and 331 to the sequence of IgG4 G2 ⁇ a in Eur J Immunol. 1999 Aug; 29(8):2613-24 ).
  • methionine at EU-numbering position 397 was mutated into valine to improve the stability of IgG2 under acidic condition.
  • SKSC SEQ ID NO: 62
  • introduction of mutations at positions 131 and 133 will generate a novel non-naturally occurring 9-amino acid peptide sequence that could be a T-cell epitope peptide, thereby causing a risk of immunogenicity.
  • the peptide sequence around positions 131 to 139 was converted into the same as IgG1 by mutating glutamic acid at EU-numbering position 137 into glycine and mutating serine at EU-numbering position 138 into glycine.
  • the constant region sequence M14 (SEQ ID NO: 129) was produced by introducing all the above mutations.
  • huPM1-M14 prepared by using huPM1-M14 as an H chain and huPM1-L (SEQ ID NO: 162) as an L chain, was carried out by the method described in Referential Example 7.
  • the prepared huPM1-MI4 (SEQ ID NO: 163), huPM1-IgG1, and huPM1-IgG2 were assessed for the heterogeneity using cation exchange chromatography by the method described in Referential Example 7.
  • the heterogeneity was also reduced in huPM1-M14 as in huPM1-SKSC.
  • huPM1 is an IgG1 antibody.
  • IgG1 antibody For the heterogeneity in the C-terminal sequence of the H chain of IgG antibody, the deletion of the C-terminal lysine residue and the amidation of the C-terminal amino group due to deletion of the two C-terminal amino acids, glycine and lysine, have been reported ( Anal Biochem. 2007 Jan 1;360(1): 75-83 ).
  • huPM1 while the major component is a sequence in which the C-terminal lysine encoded by the nucleotide sequence has been deleted by post-translational modification, there are also a minor component in which the lysine remains and a minor component in which the C-terminal amino group is amidated due to deletion of both glycine and lysine, which contribute to heterogeneity.
  • Producing a pharmaceutical in a large scale while maintaining the difference in the heterogeneity of desired/related substances between products is not easy but rather results in increase of cost, and it is thus desired that the substance be composed of a single substance as much as possible.
  • an antibody is developed as a pharmaceutical, reduction of the heterogeneity is desired.
  • the C-terminal of the H chain has no heterogeneity when developed as pharmaceuticals. It is also desirable to prolong the plasma half-life of the antibody in order to reduce the antibody dose.
  • huPM1-SKSC which has high stability and in which the above-mentioned heterogeneity related to antibodies with IgG2-isotype constant regions is reduced
  • glutamic acid at EU-numbering position 137 was substituted with glycine; serine at position 138 with glycine; histidine at position 268 with glutamine; arginine at position 355 with glutamine; and glutamine at position 419 with glutamic acid.
  • glycine and lysine at positions 446 and 447 were deleted to reduce the heterogeneity of the H-chain C terminus, thereby obtaining huPM1-M58 (SEQ ID NO: 164).
  • huPM1-M58 prepared by using huPM1-M58 as an H chain and huPM1-L (SEQ ID NO: 162) as an L chain was expressed and purified by the method described in Example 4.
  • huPM1-M58, huPM1-IgG1, and huPM1-IgG2 were assessed for the heterogeneity and stability by the methods described in Example 5 using cation exchange chromatography and DSC, respectively.
  • IgG molecule The prolonged retention (slow elimination) of IgG molecule in plasma is due to the function of FcRn, which is known as a salvage receptor of IgG molecule ( Nat Rev Immunol. 2007 Sep;7(9): 715-25 ).
  • FcRn FcRn
  • IgG molecules bind to FcRn expressed in endosomes under the acidic conditions within the endosome (approx. pH 6.0). While IgG molecules that are not bound to FcRn are transferred to and degraded in lysosomes, those bound to FcRn are translocated to the cell surface and then released from FcRn into plasma again under the neutral conditions in plasma (approx. pH 7.4).
  • IgG-type antibodies are known to include IgG1, IgG2, IgG3, and IgG4 isotypes.
  • the plasma half-lives of these isotypes in human are reported to be about 36 days for IgG1 and IgG2; about 29 days for IgG3; and 16 days for IgG4 ( Nat. Biotechnol. 2007 Dec; 25(12): 1369-72 ).
  • the retention of IgG1 and IgG2 in plasma is believed to be the longest.
  • the isotypes of antibodies used as pharmaceutical agents are IgG1, IgG2, and IgG4.
  • Reported methods for further improving the pharmacokinetics of these IgG antibodies include methods for improving the above-described binding activity to human FcRn by altering the sequence of IgG constant region ( J. Biol. Chem. 2007 Jan 19;282(3): 1709-17 ; J. Immunol. 2006 Jan 1;176(1): 346-56 ).
  • FcRn is a complex of FcRn and ⁇ 2-microglobulin.
  • Oligo-DNA primers were prepared based on the published human FcRn gene sequence ( J. Exp. Med. (1994) 180 (6), 2377-2381 ).
  • a DNA fragment encoding the whole gene was prepared by PCR using human cDNA (Human Placenta Marathon-Ready cDNA, Clontech) as a template and the prepared primers.
  • a DNA fragment encoding the extracellular domain containing the signal region was amplified by PCR, and inserted into an animal cell expression vector (the amino acid sequence of human FcRn/SEQ ID NO: 165).
  • oligo-DNA primers were prepared based on the published human ⁇ 2-microglobulin gene sequence ( Proc. Natl. Acad. Sci. U.S.A. 99 (26), 16899-16903 (2002 )).
  • a DNA fragment encoding the whole gene was prepared by PCR using human cDNA (Hu-Placenta Marathon-Ready cDNA, CLONTECH) as a template and the prepared primers.
  • human cDNA Human-Placenta Marathon-Ready cDNA, CLONTECH
  • a DNA fragment encoding the whole ⁇ 2-microglobulin containing the signal region was amplified by PCR and inserted into an animal cell expression vector (the amino acid sequence of human ⁇ 2-microglobulin/SEQ ID NO: 166).
  • Soluble human FcRn was expressed by the following procedure.
  • the prepared plasmids for human FcRn and ⁇ 2-microglobulin were introduced into the human embryonic kidney cancer-derived cell line HEK293H (Invitrogen) using 10% fetal bovine serum (Invitrogen) by lipofection.
  • the resulting culture supernatant was collected and purified using IgG Sepharose 6 Fast Flow (Amersham Biosciences) by the method described in J. Immunol. 2002 Nov 1; 169(9):5171-80 . Then further purification was carried out using HiTrap Q HP (GE Healthcare).
  • the binding to human FcRn was assessed using Biacore 3000.
  • An antibody was bound to Protein L or rabbit anti-human IgG Kappa chain antibody immobilized onto a sensor chip, human FcRn was added as an analyte for interaction with the antibody, and the affinity (KD) was calculated from the amount of bound human FcRn.
  • Protein L was immobilized onto sensor chip CM5 (BIACORE) by the amine coupling method using 50 mM Na-phosphate buffer (pH 6.0) containing 150 mM NaCl as the running buffer. Then, an antibody was diluted with the running buffer containing 0.02% Tween20, and injected and allowed to bind to the chip. Human FcRn was then injected to assess the binding activity of the antibody to the human FcRn.
  • the affinity was calculated using BIAevaluatipn software.
  • the obtained sensorgram was used to calculate the amount of hFcRn bound to the antibody immediately before the end of human FcRn injection. This was fitted by the steady state affinity method to calculate the affinity of human FcRn for the antibody.
  • binding activities of huPM1-IgG1 and huPM1-M58 to human FcRn were assessed using BIAcore. As shown in Table 19, the binding activity of huPM1-M58 was greater than that of huPM1-IgG1 by about 1.4 times. Table 19 KD( ⁇ M) huPM1-IgG1 1.62 huPM1-M58 1.17
  • mice The pharmacokinetics in human FcRn transgenic mice (B6.mFcRn-/-.hFcRn Tg line 276 +/+ mice; Jackson Laboratories) was assessed by the following procedure. An antibody was intravenously administered once at a dose of 1 mg/kg to mice, and blood was collected at appropriate time points. The collected blood was immediately centrifuged at 15,000 rpm for 15 minutes at 4°C to obtain plasma. The separated plasma was stored in a freezer at -20°C or below until use. The plasma concentration was determined by ELISA.
  • Protein A was immobilized onto all flow cells of sensor chip CM5 (GE Healthcare Bioscinences) by the amine coupling method.
  • the experiment was carried out using HBS-EP+ (10 mM HEPES, 0.15 M NaCl, 3 mM EDTA, 0.05% v/v Surfactant P20) as a running buffer at a flow rate of 10 ⁇ L/min.
  • the carboxyl groups of carboxymethyl dextran on the sensor chip were activated with 100 ⁇ L of a 1:1 mixture of 75 mg/ml EDC (N-ethyl-N'-(3-dimethylaminopropyl)carbodiimide hydrochloride) and 11.5 mg/ml NHS (N-hydroxysuccinimide), and Protein A prepared at 50 ⁇ g/ml using 10 mM acetate buffer (pH 4.5) was allowed to flow for reaction. Then, 100 ⁇ L of 1 M ethanolamine hydrochloride (pH 8.5) was allowed to flow to inactivate the unreacted active groups. Ultimately, about 4000 to 5000 RU were immobilized. The experiment was carried out at 25°C at all times.
  • the running buffer used was HBS-EP+.
  • Each antibody was prepared at 0.25 ⁇ g/ml, or prepared so that about 100 RU would bind to Protein A.
  • rhNR10 used as an analyte was prepared at 0, 38.5, 77.0, and 154 nM, or at 0, 19.25, and 77.01 nM using HBS-EP+.
  • the antibody solution was captured on Protein A, and an analyte solution was reacted at a flow rate of 20 ⁇ L/min for three minutes. Then, the solution was switched to HBS-EP+, and the dissociation phase was measured for five minutes.
  • the sensor chip was regenerated by washing with 10 mM glycine-HCl (pH 1.5). The obtained sensorgrams were kinetically analyzed using the Biacore-specific data analysis software, Biacore T100 Evaluation Software Version 1.1.
  • the anti-NR10 antibodies obtained by the present inventors exhibit an effective neutralizing activity against R10, and are useful as, for example, therapeutic agents for inflammatory diseases.

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US12122840B2 (en) 2007-09-26 2024-10-22 Chugai Seiyaku Kabushiki Kaisha Method of modifying isoelectric point of antibody via amino acid substitution in CDR

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